Viral chemokine-antigen fusion proteins

ABSTRACT

The present invention relates to a vaccine for increasing the immunogenicity of a tumor antigen thus allowing treatment of cancer, as well as a vaccine that increases the immunogenicity of a viral antigen, thus allowing treatment of viral infection, including immunodeficiency virus (HIV) infection. In particular, the present invention provides a fusion protein comprising a viral chemokine fused to either a tumor antigen or viral antigen which is administered as either a protein or nucleic acid vaccine to elicit an immune response effective in treating cancer or effective in treating or preventing viral infection.

CROSS REFERENCE TO RELATED APPLICATIONS

This is a divisional of U.S. application Ser. No. 13/009,572, filed Jan. 19, 2011, which is a continuation of U.S. application Ser. No. 10/380,927, filed Mar. 17, 2003, issued as U.S. Pat. No. 7,897,152 on Mar. 1, 2011, which is the U.S. National Stage of International Application No. PCT/US2001/029075, filed Sep. 17, 2001, which was published in English under PCT Article 21(2), and which claims the benefit of priority of U.S. Provisional Application No. 60/233,067, filed Sep. 15, 2000. All of the above-listed applications are herein incorporated by reference in their entirety.

FIELD OF THE INVENTION

The present invention relates to a vaccine for increasing the immunogenicity of a tumor antigen thus allowing treatment of cancer, as well as a vaccine that increases the immunogenicity of a viral antigen, thus allowing treatment of viral infection, including immunodeficiency virus (HIV) infection. In particular, the present invention provides a fusion protein comprising a viral chemokine fused to either a tumor antigen or viral antigen which is administered as either a protein or nucleic acid vaccine to elicit an immune response effective in treating cancer or effective in treating or preventing viral infection.

BACKGROUND OF THE INVENTION

Tumor cells are known to express tumor-specific antigens on the cell surface. These antigens are believed to be poorly immunogenic, largely because they represent gene products of oncogenes or other cellular genes which are normally present in the host and are therefore not clearly recognized as nonself. Although numerous investigators have tried to target immune responses against epitopes from various tumor specific antigens, none have been successful in eliciting adequate tumor immunity in vivo (71).

Humans are particularly vulnerable to cancer as a result of an ineffective immunogenic response (72). In fact, the poor immunogenicity of relevant cancer antigens has proven to be the single greatest obstacle to successful immunotherapy with tumor vaccines (73). Over the past 30 years, literally thousands of patients have been administered tumor cell antigens as vaccine preparations, but the results of these trials have demonstrated that tumor cell immunization has failed to provide a rational basis for the design or construction of effective vaccines. Even where patients express

tumor-specific antibodies or cytotoxic T-cells, this immune response does not correlate with a suppression of the associated disease. This failure of the immune system to protect the host may be due to expression of tumor antigens that are poorly immunogenic or to heterologous expression of specific antigens by various tumor cells. The appropriate presentation of tumor antigens in order to elicit an immune response effective in inhibiting tumor growth remains a central issue in the development of an effective cancer vaccine.

Chemokines are a group of usually small secreted proteins (7-15 kDa) induced by inflammatory stimuli and are involved in orchestrating the selective migration, diapedesis and activation of blood-born leukocytes that mediate the inflammatory response (23,26). Chemokines mediate their function through interaction with specific cell surface receptor proteins (23). At least four chemokine subfamilies have been identified as defined by a cysteine signature motif, termed CC, CXC, C and CX₃C, where C is a cysteine and X is any amino acid residue. Structural studies have revealed that at least both CXC and CC chemokines share very similar tertiary structure (monomer), but different quaternary structure (dimer) (120-124). For the most part, conformational differences are localized to sections of loop or the N-terminus.

There remains a great need for a method of presenting tumor antigens, which are known to be poorly immunogenic, “self” antigens to a subject's immune system in a manner that elicits an immune response powerful enough to inhibit the growth of tumor cells in the subject. This invention overcomes the previous limitations and shortcomings in the art by providing a fusion protein comprising a viral chemokine and a tumor antigen which can produce an in vivo immune response, resulting in the inhibition of tumor cells. There is also a continuing need for a method of presenting poorly antigenic viral antigens to a subject's immune system, particularly as relates to viral antigens such as HIV antigens. This invention also overcomes previous shortcomings in the field of viral vaccine development by providing a fusion protein comprising a viral chemokine and a viral antigen which is effective as a vaccine for treating or preventing viral infection.

SUMMARY OF THE INVENTION

The present invention provides a fusion polypeptide comprising a viral chemokine and a tumor antigen. In a preferred embodiment, the viral chemokine can be MIPI, MIPII, MIPIII, or any of the other viral chemokines set forth in Table 1, and the tumor antigen can be a 8 cell tumor antigen or MUC-1.

The present invention also provides a fusion polypeptide comprising a viral chemokine and a viral antigen. In a preferred embodiment, the viral chemokine can be MIPI, MUM, MIPIII, or any of the other viral chemokines set forth in Table 1, and the viral antigen can be an HIV antigen, such as gp120, gp160, gp41, an active fragment of gp120, an active fragment of gp160 and/or an active fragment of gp41.

In addition, the present invention provides a method of producing an immune response in a subject, comprising administering to the subject any of the fusion polypeptides of this invention, comprising a viral chemokine and viral antigen, or a viral chemokine and a tumor antigen, either as a protein or a nucleic acid encoding the fusion polypeptide.

Also provided is a method of treating a cancer in a subject comprising administering to the subject any of the fusion polypeptides of this invention, comprising a viral chemokine and a tumor antigen, either as a protein or a nucleic acid encoding the fusion polypeptide.

The invention also provides a method of treating or preventing a viral infection in a subject, comprising administering to the subject any of the fusion polypeptides of this invention, comprising a viral chemokine and a viral antigen, either as a protein or a nucleic acid encoding the fusion polypeptide.

Further provided is a method of treating or preventing HIV infection in a subject, comprising administering to the subject any of the fusion polypeptides of this invention, comprising a viral chemokine and a human immunodeficiency virus (HIV) antigen, either as a protein or a nucleic acid encoding the fusion polypeptide.

A method of treating a B cell tumor in a subject is also provided, comprising administering to the subject any of the fusion polypeptides of this invention, comprising a viral chemokine and a B cell tumor antigen, either as a protein or a nucleic acid encoding the fusion polypeptide.

Various other objectives and advantages of the present invention will become apparent from the following detailed description.

DESCRIPTION OF THE PREFERRED EMBODIMENTS

As used in the claims, “a” can include multiples. For example, “a cell” can mean a single cell or more than one cell. Also, unless otherwise indicated, all references herein to a “chemokine” refer to a viral chemokine.

The present invention is based on the unexpected discovery that the administration of a fusion protein comprising a viral chemokine and a tumor antigen or administration of a nucleic acid encoding a fusion protein comprising a viral chemokine and a tumor antigen yields an effective and specific anti-tumor immune response by converting a “self” tumor antigen into a potent immunogen by binding to a viral chemokine moiety. A further unexpected discovery of the present invention is that the viral chemokine-tumor antigen fusion polypeptide vaccine of this invention is superior to a human chemokine-tumor antigen fusion polypeptide vaccine, as it provides a more potent immune response and does not cause the production of auto-antibodies directed against the human chemokine moiety of the latter fusion polypeptide.

Thus, the present invention provides a fusion polypeptide comprising a viral chemokine and a tumor antigen. The fusion polypeptide can be present in a purified form and can induce an immune response against the tumor antigen and inhibit the growth of tumor cells expressing the tumor antigen. “Purified” as used herein means the polypeptide is sufficiently free of contaminants or cell components with which proteins normally occur to allow the peptide to be used therapeutically. It is not contemplated that “purified” necessitates having a preparation that is technically totally pure (homogeneous), but purified as used herein means the fusion polypeptide is sufficiently pure to provide the polypeptide in a state where it can be used therapeutically. As used herein, “fusion polypeptide” means a polypeptide made up of two or more amino acid sequences representing peptides or polypeptides from different sources. Also as used herein, “epitope” refers to a specific amino acid sequence of limited length which, when present in the proper conformation, provides a reactive site for an antibody or T cell receptor. The identification of epitopes on antigens can be carried out by immunology protocols that are standard in the art (74). As further used herein, “tumor antigen” describes a polypeptide expressed on the cell surface of specific tumor cells and which can serve to identify the type of tumor. An epitope of the tumor antigen can be any site on the antigen that is reactive with an antibody or T cell receptor.

As used herein, “viral chemokine” means a protein encoded by a virus which orchestrates a chemotactic response typically after binding to specific O-protein-coupled cell surface receptors on target cells (e.g., antigen presenting cells (APC), such as dendritic cells, monocytes, macrophages, keratinocytes and B cells), comprising the selective migration, diapedesis and activation of leukocytes which mediate the inflammatory response.

Numerous viral chemokines have been identified, including, for example, chemokines produced by Kaposi's sarcoma-associated herpes virus (KSHV/HHV8), which are analogues of human chemokine MIP-1s. These are designated VMS % vMIPII and vMIPIII. (128, 129). vMIPI is an agonist chemokine which binds to CCR8-expressing cells, e.g., T helper 2 (T_(H)2) cells, while vMIPII is considered to be a broad spectrum antagonist of chemotaxis, and binds to several chemokine receptors such as CCR1, CCR2, CCR5, CXCR4, and cytomegalovirus chemokine receptor US 28. vMIPII can induce chemotaxis via binding to CCR3 and CCR8. vMIPIII is an agonist which binds CCR4 expressed by T_(H)2-type T cells.

The viral chemokine of this invention can include, but is not limited to, vMIPI, vMIPII, vMIPIII, and any of the viral chemokines set forth in Table 1 as well as any other viral chemokine now known or later identified (128). Additional examples of viral chemokines which may be used in the compositions and methods of the present invention are set forth in Lalani et al. (Immunology Today 21:100-106 (2000)), the contents of which are hereby incorporated by reference in their entirety.

It will be appreciated by one of skill in the art that viral chemokines can include active fragments of viral chemokines which retain the activity, including chemotaxis and inhibition of chemotaxis, of the intact molecule.

A viral chemokine consists of two structural portions: the amino terminal portion and the carboxy terminal portion. The amino terminal portion is responsible for viral chemokine receptor binding and the carboxy terminal end binds to heparin and heparin sulfate, for example, in the extracellular matrix and on the surface of endothelial cells. The viral chemokine gene can be fragmented as desired and the fragments can be fused to a specific marker gene encoding an antigen (e.g., Muc-1 VNT, lymphoma scFv, etc.). The fusion polypeptide comprising the viral chemokine fragment and the tumor or viral antigen can be produced and purified as described herein and tested for immunogenicity according to the methods provided herein. By producing several fusion polypeptides having viral chemokine fragments of varying size, the minimal size chemokine fragment which imparts an immunological effect can be identified.

The tumor antigen moiety of the fusion polypeptide of this invention can be any tumor antigen now known or later identified as a tumor antigen. The appropriate tumor antigen used in the fusion polypeptide naturally depends on the tumor type being treated. For example, the tumor antigen can be, but is not limited to human epithelial cell mucin (Muc-1; a 20 amino acid core repeat for Muc-1 glycoprotein, present on breast cancer cells and pancreatic cancer cells), the Ha-ras oncogene product, p53, carcino-embryonic antigen (CEA), the raf oncogene product, GD2, GD3, GM2, TF, sTn, MAGE-1, MAGE-3, tyrosinase, gp75, Melan-A/Mart-1, gp100, HER2/neu, EBV-LMP 1 & 2, HPV-F4, 6, 7, prostatic serum antigen (PSA), alpha-fetoprotein (AFP), CO17-1A, GA733, gp72, p53, the ras oncogene product, proteinase 3, Wilm's tumor antigen-1, telomerase, HPV E7 and melanoma gangliosides, as well as any other tumor antigens now known or identified in the future. Tumor antigens can be obtained following known procedures or are commercially available (79). The effectiveness of the fusion protein in eliciting an immune response against a particular tumor antigen can be determined according to methods standard in the art for determining the efficacy of vaccines and according to the methods set forth in the Examples.

Additionally, the tumor antigen of the present invention can be an antibody which can be produced by a B cell tumor (e.g., B cell lymphoma; B cell leukemia; myeloma) or the tumor antigen can be a fragment of such an antibody, which contains an epitope of the idiotype of the antibody. The epitope fragment can comprise as few as nine amino acids. For example, the tumor antigen of this invention can be a malignant B cell antigen receptor, a malignant B cell immunoglobulin idiotype, a variable region of an immunoglobulin, a hypervariable region or complementarity determining region (CDR) of a variable region of an immunoglobulin, a malignant T cell receptor (TCR), a variable region of a TCR and/or a hypervariable region of a TCR.

In a preferred embodiment, the tumor antigen of this invention can be a single chain antibody (scFv), comprising linked V_(H) and V_(L) domains and which retains the conformation and specific binding activity of the native idiotype of the antibody (27). Such single chain antibodies are well known in the art and can be produced by standard methods and as described in the Examples herein.

In addition, the tumor antigen of the present invention can be an epitope of the idiotype of a T cell receptor, which can be produced by a T cell tumor (e.g., T cell lymphoma; T cell leukemia; myeloma). The epitope can comprise as few as nine amino acids.

As will be appreciated by those skilled in the art, the invention also includes peptides and polypeptides having slight variations in amino acid sequences or other properties. Such variations may arise naturally as allelic variations (e.g., due to genetic polymorphism) or may be produced by human intervention (e.g., by mutagenesis of cloned DNA sequences), such as induced point, deletion, insertion and substitution mutantions. Minor changes in amino acid sequence are generally preferred, such as conservative amino acid replacements, small internal deletions or insertions, and additions or deletions at the ends of the molecules. Substitutions may be designed based on, for example, the model of Dayhoff et al. (80). These modifications can result in changes in the amino acid sequence, provide silent mutations, modify a restriction site, or provide other specific mutations.

The fusion polypeptides can comprise one or more selected epitopes on the same tumor antigen, one or more selected epitopes on different tumor antigens, as well as repeats of the same epitope, either in tandem or interspersed along the amino acid sequence of the fusion polypeptide. The tumor antigen can be positioned in the fusion polypeptide at the carboxy terminus of the viral chemokine, the amino terminus of viral chemokine and/or at one or more internal sites within the viral chemokine amino acid sequence. Additionally, the fusion polypeptide can comprise more than one viral chemokine in any combination and in any order with the various tumor antigens described above.

It would be routine for an artisan to produce a fusion protein comprising any viral chemokine region and any human tumor antigen (e.g., human single chain antibody) region according to the methods described herein, on the basis of the availability in the art of the nucleic acid and/or amino acid sequence of the viral chemokine of interest and the human tumor antigen of interest.

The present invention further provides a fusion polypeptide comprising a first region comprising a viral chemokine selected from the group consisting of vMIPI, vMIPII and vMIPIII, and a second region comprising a tumor antigen selected from the group consisting of human epithelial cell mucin (Muc-1), the Ha-ras oncogene product, p53, carcino-embryonic antigen (CEA), the raf oncogene product, GD2, GD3, GM2, TF, sTn, MAGE-1, MAGE-3, tyrosinase, gp75, Melan-A/Mart-1, gp100, HER2/neu, EBV-LMP 1 & 2, HPV-F4, 6, 7, prostatic serum antigen (PSA), alpha-fetoprotein (AFP), CO17-1A, GA733, gp72, p53, the ras oncogene product, HPV E7, melanoma gangliosides, an antibody produced by a B cell tumor (e.g., B cell lymphoma; B cell leukemia; myeloma), a fragment of such an antibody, which contains an epitope of the idiotype of the antibody, a malignant B cell antigen receptor, a malignant B cell immunoglobulin idiotype, a variable region of an immunoglobulin, a hypervariable region or CDR of a variable region of an immunoglobulin, a malignant T cell receptor (TCR), a variable region of a TCR and/or a hypervariable region of a TCR.

For example, the present invention provides a fusion polypeptide comprising an scFv cloned from a human subject's biopsy tumor material or from a hybridoma cell line producing a lymphoma antibody and a viral chemokine moiety (e.g., vMIPI, vMIPII, vMIPIII, etc.). In addition, the present invention provides a viral chemokine fused with the Muc-1 core epitope of human breast cancer or human pancreatic cancer. Muc-1 is a glycoprotein (Mr>200,000) abundantly expressed on breast cancer cells and pancreatic tumor cells. A variable number of tandem (VNT) repeats of a 20 amino acid peptide (PDTRPAPGSTAPPAHGVTSA; SEQ ID NO:1) include B and T cell epitopes. Thus, the present invention provides a fusion protein comprising vMIPI and Muc-1 VNT and vMIPII and Muc-1 VNT. The expression vector is designed so that a VNT can be changed by routine cloning methods to produce a fusion polypeptide comprising vMIPI or vMIPI™ fused with a Muc-1 VNT dimer, trimer, tetramer, pentamer, hexamer, etc.

In specific embodiments, the present invention also provides a fusion polypeptide comprising vMIPI and human Muc-1, a fusion polypeptide comprising vMIPII and human Muc-1, and a fusion polypeptide comprising vMIPIII and human Muc-1 and human Muc-1.

The present invention further provides a fusion polypeptide comprising a viral chemokine (e.g., vMIPI, vMIPII, vMIPIII, etc.) and a scFv which recognizes tumor antigens, such as idiotype-specific scFv, Muc-1, etc. Such a fusion polypeptide would allow migration, recruitment and activation of specialized cells of the immune system, such as natural killer (NK) cells, macrophages, dendritic cells (DC), polymorphonuclear (PMN) leukocytes, cytotoxic lymphocytes (CTL), etc., which would destroy the target cell.

The fusion polypeptide of this invention can further comprise a spacer sequence between the viral chemokine and the tumor antigen or viral antigen, which can have the amino acid sequence EFNDAQAPKSLE (SEQ ID NO:2), or an amino acid sequence with conservative substitutions such that it has the same functional activity as the amino acid sequence of SEQ ID NO:2, which allows for retention of the correct folding of the tumor antigen region of the polypeptide.

In addition, the present invention provides a composition comprising the fusion polypeptide of this invention and a suitable adjuvant. Such a composition can be in a pharmaceutically acceptable carrier, as described herein. As used herein, “suitable adjuvant” describes a substance capable of being combined with the fusion polypeptide to enhance an immune response in a subject without deleterious effect on the subject. A suitable adjuvant can be, but is not limited to, for example, an immunostimulatory cytokine, SYNTEX adjuvant formulation 1 (SAF-1) composed of 5 percent (wt/vol) squalene (DASF, Parsippany, N.J.), 2.5 percent Pluronic, L121 polymer (Aldrich Chemical, Milwaukee), and 0.2 percent polysorbate (Tween 80, Sigma) in phosphate-buffered saline. Other suitable adjuvants are well known in the art and include QS-21, Freund's adjuvant (complete and incomplete), alum, aluminum phosphate, aluminum hydroxide, N-acetyl-muramyl-L-threonyl-D-isoglutamine (thr-MDP), N-acetyl-nor-muramyl-L-alanyl-D-isoglutamine (CGP 11637, referred to as nor-MDP), N-acetylmuramyl-L-alanyl-D-isoglutaminyl-L-alanine-2-(1′-2′-dipalmitoyl-sn-glycero-3-hydroxyphosphoryloxy)-ethylamine (CGP 19835A, referred to as MTP-PE) and RIK which contains three components extracted from bacteria, monophosphoryl lipid A, trealose dimycolate and cell wall skeleton (MPL+TDM+CWS) in 2% squalene/Tween 80 emulsion.

The adjuvant, such as an immunostimulatory cytokine can be administered before the administration of the fusion protein or nucleic acid encoding the fusion protein, concurrent with the administration of the fusion protein or nucleic acid or up to five days after the administration of the fusion polypeptide or nucleic acid to a subject. QS-21, similarly to alum, complete Freund's adjuvant, SAF, etc., can be administered within hours of administration of the fusion protein or nucleic acid.

Furthermore, combinations of adjuvants, such as immunostimulatory cytokines can be co-administered to the subject before, after or concurrent with the administration of the fusion polypeptide or nucleic acid. For example, combinations of adjuvants, such as immunostimulatory cytokines, can consist of two or more of immunostimulatory cytokines of this invention, such as GM/CSF, interleukin-2, interleukin-12, interferon-gamma, interleukin-4, tumor necrosis factor-alpha, interleukin-1, hematopoietic factor flt3L, CD40L, B7.1 co-stimulatory molecules and B7.2 co-stimulatory molecules. The effectiveness of an adjuvant or combination of adjuvants may be determined by measuring the immune response directed against the fusion polypeptide with and without the adjuvant or combination of adjuvants, using standard procedures, as described herein.

Furthermore, the present invention provides a composition comprising the fusion polypeptide of this invention or a nucleic acid encoding the fusion polypeptide of this invention and an adjuvant, such as an immunostimulatory cytokine or a nucleic acid encoding an adjuvant, such as an immunostimulatory cytokine. Such a composition can be in a pharmaceutically acceptable carrier, as described herein. The immuno-stimulatory cytokine used in this invention can be, but is not limited to, GM/CSF, interleukin-2, interleukin-12, interferon-gamma, interleukin-4, tumor necrosis factor-alpha, interleukin-1, hematopoietic factor flt3L, CD40L, B7.1 con-stimulatory molecules and B7.2 co-stimulatory molecules.

The present invention further contemplates a fusion polypeptide comprising a viral chemokine, or active fragment thereof, as described herein and a viral antigen, which can be, for example, an antigen of human immunodeficiency virus (HIV). An 111V antigen of this invention can be, but is not limited to, the envelope glycoprotein gp120, the third hypervariable region of the envelope glycoprotein, gp120 of HIV-1 (the disulfate loop V3), having the amino acid sequence: NCTRPNNNTRKRTRIQRGPGRA FVTIGKIGNMRQAHCNIS (SEQ ID NO:3), any other antigenic fragment of gp120, the envelope glycoprotein gp160, an antigenic fragment of gp160, the envelope glycoprotein gp41 and/or an antigenic fragment of gp41. For example, the nucleic acid encoding the V3 loop can be fused to the 3′ end of the nucleic acid encoding a viral chemokine (e.g., vMIPI, vMIPII, or vMIPIII) directly or separated by nucleic acid encoding a spacer sequence. The viral chemokine-V3 loop fusion polypeptide can be produced in an expression system as described herein and purified as also described herein.

In specific embodiments, the present invention provides a fusion polypeptide comprising a viral chemokine and a human immunodeficiency virus (HIV) antigen, wherein the viral chemokine can be vMIPI, vMIPII, vMIPIII, or any other viral chemokine, and wherein the HIV antigen can be gp120, gp160, gp41, an active (i.e., antigenic) fragment of gp120, an active antigenic) fragment of gp160 and an active (i.e., antigenic) fragment of gp41.

Further provided in this invention is fusion polypeptide comprising vMIPI and HIV gp120, a fusion polypeptide comprising vMIPII and HIV gp120, and a fusion polypeptide comprising vMIPIII and HIV gp120.

An isolated nucleic acid encoding the fusion polypeptides of this invention as described above is also provided. By “isolated nucleic acid” is meant a nucleic acid molecule that is substantially free of the other nucleic acids and other components commonly found in association with nucleic acid in a cellular environment. Separation techniques for isolating nucleic acids from cells are well known in the art and include phenol extraction followed by ethanol precipitation and rapid solubilization of cells by organic solvent or detergents (81).

The nucleic acid encoding the fusion polypeptide can be any nucleic acid that functionally encodes the fusion polypeptide. To functionally encode the polypeptide (i.e., allow the nucleic acid to be expressed), the nucleic acid can include, for example, expression control sequences, such as an origin of replication, a promoter, an enhancer and necessary information processing sites, such as ribosome binding sites, RNA splice sites, polyadenylation sites and transcriptional terminator sequences. Preferred expression control sequences are promoters derived from metallothionine genes, actin genes, immunoglobulin genes, CMV, SV40, adenovirus, bovine papilloma virus, etc. A nucleic acid encoding a selected fusion polypeptide can readily be determined based upon the genetic code for the amino acid sequence of the selected fusion polypeptide and many nucleic acids will encode any selected fusion polypeptide. Modifications in the nucleic acid sequence encoding the fusion polypeptide are also contemplated. Modifications that can be useful are modifications to the sequences controlling expression of the fusion polypeptide to make production of the fusion polypeptide inducible or repressible as controlled by the appropriate inducer or repressor. Such means are standard in the art (81). The nucleic acids can be generated by means standard in the art, such as by recombinant nucleic acid techniques, as exemplified in the examples herein and by synthetic nucleic acid synthesis or in vitro enzymatic synthesis.

A vector comprising any of the nucleic acids of the present invention and a cell comprising any of the vectors of the present invention are also provided. The vectors of the invention can be in a host (e.g., cell line or transgenic animal) that can express the fusion polypeptide contemplated by the present invention.

There are numerous E. coli (Escherichia coli) expression vectors known to one of ordinary skill in the art useful for the expression of nucleic acid encoding proteins such as fusion proteins. Other microbial hosts suitable for use include bacilli, such as Bacillus subtilis, and other enterobacteria, such as Salmonella, Serratia, as well as various Pseudomonas species. These prokaryotic hosts can support expression vectors which will typically contain expression control sequences compatible with the host cell (e.g., an origin of replication). In addition, any number of a variety of well-known promoters will be present, such as the lactose promoter system, a tryptophan (Trp) promoter system, a beta-lactamase promoter system, or a promoter system from phage lambda. The promoters will typically control expression, optionally with an operator sequence and have ribosome binding site sequences for example, for initiating and completing transcription and translation. If necessary, an amino terminal methionine can be provided by insertion of a Met codon 5′ and in-frame with the protein. Also, the carboxy-terminal extension of the protein can be removed using standard oligonucleotide mutagenesis procedures.

Additionally, yeast expression can be used. There are several advantages to yeast expression systems. First, evidence exists that proteins produced in a yeast secretion system exhibit correct disulfide pairing. Second, post-translational glycosylation is efficiently carried out by yeast secretory systems. The Saccharomyces cerevisiae pre-pro-alpha-factor leader region (encoded by the MFα-1 gene) is routinely used to direct protein secretion from yeast (82). The leader region of pre-pro-alpha-factor contains a signal peptide and a pro-segment which includes a recognition sequence for a yeast protease encoded by the KEX2 gene. This enzyme cleaves the precursor protein on the carboxyl side of a Lys-Arg dipeptide cleavage-signal sequence. The polypeptide coding sequence can be fused in-frame to the pre-pro-alpha-factor leader region. This construct is then put under the control of a strong transcription promoter, such as the alcohol dehydrogenase I promoter or a glycolytic promoter. The protein coding sequence is followed by a translation termination codon which is followed by transcription termination signals. Alternatively, the polypeptide coding sequence of interest can be fused to a second protein coding sequence, such as Sj26 or β-galactosidase, used to facilitate purification of the fusion protein by affinity chromatography. The insertion of protease cleavage sites to separate the components of the fusion protein is applicable to constructs used for expression in yeast.

Efficient post-translational glycosylation and expression of recombinant proteins can also be achieved in Baculovirus systems in insect cells.

Mammalian cells permit the expression of proteins in an environment that favors important post-translational modifications such as folding and cysteine pairing, addition of complex carbohydrate structures and secretion of active protein. Vectors useful for the expression of proteins in mammalian cells are characterized by insertion of the protein coding sequence between a strong viral promoter and a polyadenylation signal. The vectors can contain genes conferring either gentamicin or methotrexate resistance for use as selectable markers. The antigen and immunoreactive fragment coding sequence can be introduced into a Chinese hamster ovary (CHO) cell line using a methotrexate resistance-encoding vector. Presence of the vector RNA in transformed cells can be confirmed by Northern blot analysis and production of a cDNA or opposite strand RNA corresponding to the protein coding sequence can be confirmed by Southern and Northern blot analysis, respectively. A number of other suitable host cell lines capable of secreting intact proteins have been developed in the art and include the CHO cell lines, HeLa cells, myeloma cell lines, Jurkat cells and the like. Expression vectors for these cells can include expression control sequences, as described above.

The vectors containing the nucleic acid sequences of interest can be transferred into the host cell by well-known methods, which vary depending on the type of cell host. For example, calcium chloride transfection is commonly utilized for prokaryotic cells, whereas calcium phosphate treatment, lipofection or electroporation may be used for other cell hosts.

Alternative vectors for the expression of protein in mammalian cells, similar to those developed for the expression of human gamma-interferon, tissue plasminogen activator, clotting Factor VIII, hepatitis B virus surface antigen, protease Nexini, and eosinophil major basic protein, can be employed. Further, the vector can include CMV promoter sequences and a polyadenylation signal available for expression of inserted nucleic acid in mammalian cells (such as COS7).

The nucleic acid sequences can be expressed in hosts after the sequences have been positioned to ensure the functioning of an expression control sequence. These expression vectors are typically replicable in the host organisms either as episomes or as an integral part of the host chromosomal DNA. Commonly, expression vectors can contain selection markers, e.g., tetracycline resistance or hygromycin resistance, to permit detection and/or selection of those cells transformed with the desired nucleic acid sequences (83).

Additionally, the fusion polypeptides and/or nucleic acids of the present invention can be used in in vitro diagnostic assays, as well as in screening assays for identifying unknown tumor antigen epitopes and fine mapping of tumor antigen epitopes.

Also provided is a method for producing a fusion polypeptide comprising a viral chemokine, or an active fragment thereof and a tumor antigen or viral antigen, comprising cloning into an expression vector a first DNA fragment encoding a viral chemokine or active fragment thereof and a second DNA fragment encoding a tumor antigen or viral antigen; and expressing the DNA of the expression vector in an expression system under conditions whereby the fusion polypeptide is produced. The expression vector and expression system can be of any of the types as described herein. The cloning of the first and second DNA segments into the expression vector and expression of the DNA under conditions which allow for the production of the fusion protein of this invention can be carried out as described in the Examples section included herein. The method of this invention can further comprise the step of isolating and purifying the fusion polypeptide, according to methods well known in the art and as described herein.

Any of the fusion polypeptides, the nucleic acids and the vectors of the present invention can be in a pharmaceutically acceptable carrier and in addition, can include other medicinal agents, pharmaceutical agents, carriers, diluents, adjuvants (e.g., immunostimulatory cytokines), etc. By “pharmaceutically acceptable” is meant a material that is not biologically or otherwise undesirable, i.e., the material may be administered to an individual along with the selected antigen without causing substantial deleterious biological effects or interacting in a deleterious manner with any of the other components of the composition in which it is contained. Actual methods of preparing such dosage forms are known, or will be apparent, to those skilled in this art (84).

Thus, the present invention further provides a method for inducing an immune response in a subject capable of induction of an immune response and preferably human, comprising administering to the subject an immune response-inducing amount of the fusion polypeptide of this invention. As used herein, “an immune response-inducing amount” is that amount of fusion polypeptide which is capable of producing in a subject a humoral and/or cellular immune response capable of being detected by standard methods of measurement, such as, for example, as described herein. For example, the antigenic polypeptide region can induce an antibody response. The antibodies can treat or prevent a pathological or harmful condition in the subject in which the antibodies are produced or the antibodies can be removed from the subject and administered to another subject to treat or prevent a pathological or harmful condition. The fusion polypeptide can also induce an effector T cell (cellular) immune response which is effective in treating or preventing a pathological or harmful conditions in the subject.

In an embodiment wherein the antigen moiety of the fusion polypeptide comprises an immunoglobulin light or heavy chain or a single chain antibody, the immune response can be the production in the subject of anti-idiotype antibodies, which represent the image of the original antigen and can function in a vaccine preparation to induce an immune response to a pathogenic antigen, thereby avoiding immunization with the antigen itself (85). The anti-idiotype antibodies can treat or prevent a pathological or harmful condition in the subject in which the anti-idiotype antibodies are produced or the anti-idiotype antibodies can be removed from the subject and administered to another subject to treat or prevent a pathological or harmful condition.

Further provided is a method for inhibiting the growth of tumor cells in a subject, comprising administering to the subject a tumor cell growth-inhibiting amount of the fusion polypeptide of this invention. The subject of this method can be any subject in which a humoral and/or cellular immune response to a tumor can be induced, which is preferably an animal and most preferably a human. As used herein, “inhibiting the growth of tumor cells” means that, following administration of the fusion polypeptide, a measurable humoral and/or cellular immune response against the tumor cell epitope is elicited in the subject, resulting in the inhibition of growth of tumor cells present in the subject. The humoral immune response can be measured by detection, in the serum of the subject, of antibodies reactive with the epitope of the tumor antigen present on the fusion polypeptide, according to protocols standard in the art, such as enzyme linked immunosorbent immunoassay (ELISA) and Western blotting protocols. The cellular immune response can be measured by, for example, footpad swelling in laboratory animals, peripheral blood lymphocyte (PBL) proliferation assays and PBL cytotoxicity assays, as would be known to one of ordinary skill in the art of immunology and particularly as set forth in the available handbooks and texts of immunology protocols (86).

The present invention also provides a method of treating cancer in a subject diagnosed with cancer, comprising administering to the subject an effective amount of the fusion polypeptide of the present invention. The cancer can be, but is not limited to B cell lymphoma, T cell lymphoma, myeloma, leukemia, breast cancer, pancreatic cancer, colon cancer, lung cancer, renal cancer, liver cancer, prostate cancer, melanoma and cervical cancer.

Further provided is a method of treating a B cell tumor in a subject diagnosed with a B cell tumor, comprising administering an effective amount of the fusion polypeptide of this invention, which comprises an antibody or a fragment thereof, as described herein, in a pharmaceutically acceptable carrier, to the subject.

In specific embodiments, the present invention also provides a method of producing an immune response in a subject, comprising administering to the subject a composition comprising a fusion polypeptide of this invention and a pharmaceutically acceptable carrier and wherein the fusion polypeptide can be a fusion polypeptide comprising vMIPI and human Muc-1, a fusion polypeptide comprising vMIPII and human Muc-1 or a fusion protein comprising vMIPIII and human Muc-1.

Also provided is a method of producing an immune response in a subject, comprising administering to the subject a composition comprising a nucleic acid encoding a fusion polypeptide of this invention and a pharmaceutically acceptable carrier and wherein the fusion polypeptide is a fusion polypeptide comprising comprising vMIPI and human Muc-1, a fusion polypeptide comprising vMIPII and human Muc-1, or a fusion protein comprising vMIPIII and human Muc-1, under conditions whereby the nucleic acid of the composition can be expressed, thereby producing an immune response in the subject.

In further embodiments, the present invention also provides a method of producing an immune response in a subject, comprising administering to the subject a composition comprising a fusion polypeptide of this invention and a pharmaceutically acceptable carrier and wherein the fusion polypeptide can be a fusion polypeptide comprising vMIPI and HIV gp120, or a fusion polypeptide comprising vMIPII and HIV gp120, or a fusion polypeptide comprising vMIPIII and HIV gp120, thereby producing an immune response in the subject.

Also provided is a method of producing an immune response in a subject, comprising administering to the subject a composition comprising a nucleic acid encoding a fusion polypeptide of this invention and a pharmaceutically acceptable carrier and wherein the fusion polypeptide is a fusion polypeptide comprising vMIPI and HIV gp120, a fusion polypeptide comprising vMIPII and HIV gp120, or a fusion polypeptide comprising vMIPIII and HIV gp120 under conditions whereby the nucleic acid of the composition can be expressed, thereby producing an immune response in the subject.

Also provided is a method of producing an immune response in a subject, comprising administering to the subject a composition comprising a fusion polypeptide and a pharmaceutically acceptable carrier and wherein the fusion polypeptide is a fusion polypeptide comprising a viral chemokine and a human immunodeficiency virus (HIV) antigen, wherein the chemokine can be vMIPI, vMIPII, vMIPIII, or any other viral chemokine, and wherein the HIV antigen can be gp120, gp160, gp41, an active (i.e., antigenic) fragment of gp120, an active (i.e., antigenic) fragment of gp160 and/or an active (i.e., antigenic) fragment of gp41, thereby producing an immune response in the subject.

The present invention also provides a method of producing an immune response in a subject, comprising administering to the subject a composition comprising a nucleic acid encoding a fusion polypeptide comprising a viral chemokine and a human immunodeficiency virus (HIV) antigen, wherein the viral chemokine can be vMIPI, vMIPII, or any other vMIPIII viral chemokine, and wherein the HIV antigen can be gp120, gp160, gp41, an active (i.e., antigenic) fragment of gp120, an active (i.e., antigenic) fragment of gp160 and/or an active (i.e., antigenic) fragment of gp41, and a pharmaceutically acceptable carrier, under conditions whereby the nucleic acid can be expressed, thereby producing an immune response in the subject.

In any of the methods provided herein which recite the production of an immune response, the immune response can be humoral and/or an effector T cell (cellular) immune response, as determined according to methods standard in the alt.

In another embodiment, the present invention provides a method of treating a cancer in a subject comprising administering to the subject a composition comprising a fusion polypeptide of this invention and a pharmaceutically acceptable carrier and wherein the fusion polypeptide is a fusion polypeptide comprising vMIPI and human Muc-1, a fusion polypeptide comprising vMIPII and human Muc-1, or a fusion polypeptide comprising vMIPIII and human Muc-1, thereby treating a cancer in the subject.

Additionally provided is a method of treating a cancer in a subject, comprising administering to the subject a composition comprising a nucleic acid encoding a fusion polypeptide of this invention and a pharmaceutically acceptable carrier and wherein the fusion polypeptide is a fusion polypeptide comprising vMIPI and human Muc-1, or a fusion polypeptide comprising vMIPII and human Muc-1, or a fusion polypeptide comprising vMIPIII and human Muc-1, under conditions whereby the nucleic acid of the composition can be expressed, thereby treating a cancer in the subject.

Further provided is a method of treating or preventing HIV infection in a subject, comprising administering to the subject a composition comprising a viral chemokine and a human immunodeficiency virus (HIV) antigen, wherein the viral chemokine can be vMIPI, vMIPII, vMIPIII, or any other viral chemokine, and wherein the HIV antigen can be gp120, gp160, gp41, an active (i.e., antigenic) fragment of gp120, an active (i.e., antigenic) fragment of gp160 and/or an active (i.e., antigenic) fragment of gp41, and a pharmaceutically acceptable carrier, thereby treating or preventing HIV infection in the subject.

In addition, a method of treating or preventing HIV infection in a subject is provided herein, comprising administering to the subject a composition comprising a nucleic acid encoding a fusion polypeptide comprising a viral chemokine and a human immunodeficiency virus (HIV) antigen, wherein the viral chemokine can be vMIPI, vMIPII, vMIPIII, or any other viral chemokine, and wherein the HIV antigen can be gp120, gp160, gp41, an active (i.e., antigenic) fragment of gp120, an active (i.e., antigenic) fragment of gp160 and/or an active (i.e., antigenic) fragment of gp41, and a pharmaceutically acceptable carrier, under conditions whereby the nucleic acid can be expressed, thereby treating or preventing HIV infection in the subject.

Further provided is a method of treating or preventing HIV infection in a subject, comprising administering to the subject a composition comprising a fusion polypeptide comprising vMIPI and HIV gp120, a fusion polypeptide comprising vMIPII and HIV gp120, or a fusion polypeptide comprising vMIPIII and HIV gp120, and a pharmaceutically acceptable carrier, thereby treating or preventing HIV infection in the subject.

In addition, a method of treating or preventing HIV infection in a subject is provided herein, comprising administering to the subject a composition comprising a nucleic acid encoding a fusion polypeptide comprising vMIPI and HIV gp120, a fusion polypeptide comprising vMIPII and HIV gp120, or a fusion polypeptide comprising vMIPIII and HIV gp120, and a pharmaceutically acceptable carrier, under conditions whereby the nucleic acid can be expressed, thereby treating or preventing HIV infection in the subject.

In a further embodiment, the present invention provides a method of treating a B cell tumor in a subject, comprising administering to the subject a fusion polypeptide comprising a viral chemokine and a B cell tumor antigen, wherein the B cell tumor antigen can be an antibody, a single chain antibody or an epitope of an idiotype of an antibody, and wherein the viral chemokine can be vMIPI, vMIPII, vMIPIII, or any other viral chemokine, thereby treating a B cell tumor in the subject.

Also provided is a fusion polypeptide comprising the viral chemokine vMIPI, vMIPII, or vMIPIII and the V3 loop of HIV-1 envelope glycoprotein, gp120, as well as a fusion protein comprising vMIPI, vMIPII, or vMIPIII and gp160 of HIV-1, a fusion protein comprising vMIPI, vMIPII, or vMIPIII and gp41 of HIV-1, a fusion protein comprising vMIPI, vMIPII, or vMIPIII and an active fragment of gp120, a fusion protein comprising vMIPI, vMIPII, or vMIPIII and an active fragment of gp160 and a fusion polypeptide comprising vMIPI, vMIPII, or vMIPIII and an active fragment of gp41.

The methods of this invention comprising administering the fusion protein of this invention to a subject can further comprise the step of administering one or more adjuvants, such as an immunostimulatory cytokine to the subject. The adjuvant or adjuvants can be administered to the subject prior to, concurrent with and/or after the administration of the fusion protein as described herein.

The subject of the present invention can be any animal in which cancer can be treated by eliciting an immune response to a tumor antigen. In a preferred embodiment, the animal is a mammal and most preferably is a human.

To determine the effect of the administration of the fusion polypeptide on inhibition of tumor cell growth in laboratory animals, the animals can either be pre-treated with the fusion polypeptide and then challenged with a lethal dose of tumor cells, or the lethal dose of tumor cells can be administered to the animal prior to receipt of the fusion polypeptide and survival times documented. To determine the effect of administration of the fusion polypeptide on inhibition of tumor cell growth in humans, standard clinical response parameters can be analyzed.

To determine the amount of fusion polypeptide which would be an effective tumor cell growth-inhibiting amount, animals can be treated with tumor cells as described herein and varying amounts of the fusion polypeptide can be administered to the animals. Standard clinical parameters, as described herein, can be measured and that amount of fusion polypeptide effective in inhibiting tumor cell growth can be determined. These parameters, as would be known to one of ordinary skill in the art of oncology and tumor biology, can include, but are not limited to, physical examination of the subject, measurements of tumor size, X-ray studies and biopsies.

The present invention further provides a method for treating or preventing HIV infection in a human subject, comprising administering to the subject an HIV replication-inhibiting amount of the viral chemokines antigen fusion polypeptide of this invention. As used herein, “a replication-inhibiting amount” is that amount of fusion polypeptide which produces a measurable humoral and/or effector T cell (cellular) immune response in the subject against the viral antigen, as determined by standard immunological protocols, resulting in the inhibition of HIV replication in cells of the subject, as determined by methods well known in the art for measuring HIV replication, such as viral load measurement, which can be determined by quantitative PCR (QPCR) and branched DNA (bDNA) analysis; reverse transcriptase activity measurement, in situ hybridization, Western immunoblot, ELISA and p24 gag measurement (87,88,89,90,91). The fusion polypeptide can be administered to the subject in varying amounts and the amount of the fusion polypeptide optimally effective in inhibiting HIV replication in a given subject can be determined as described herein.

The fusion polypeptide of this invention can be administered to the subject orally or parenterally, as for example, by intramuscular injection, by intraperitoneal injection, topically, transdermally, injection directly into the tumor, or the like, although subcutaneous injection is typically preferred. Immunogenic, tumor cell growth inhibiting and HIV replication inhibiting amounts of the fusion polypeptide can be determined using standard procedures, as described. Briefly, various doses of the fusion polypeptide are prepared, administered to a subject and the immunological response to each dose is determined (92). The exact dosage of the fusion polypeptide will vary from subject to subject, depending on the species, age, weight and general condition of the subject, the severity of the cancer or HIV infection that is being treated, the particular antigen being used, the mode of administration, and the like. Thus, it is not possible to specify an exact amount. However, an appropriate amount may be determined by one of ordinary skill in the art using only routine screening given the teachings herein.

Generally, the dosage of fusion protein will approximate that which is typical for the administration of vaccines, and typically, the dosage will be in the range of about 1 to 500 μg of the fusion polypeptide per dose, and preferably in the range of 50 to 250 μg of the fusion polypeptide per dose. This amount can be administered to the subject once every other week for about eight weeks or once every other month for about six months. The effects of the administration of the fusion polypeptide can be determined starting within the first month following the initial administration and continued thereafter at regular intervals, as needed, for an indefinite period of time.

For oral administration of the fusion polypeptide of this invention, fine powders or granules may contain diluting, dispersing, and/or surface active agents, and may be presented in water or in a syrup, in capsules or sachets in the dry state, or in a nonaqueous solution or suspension wherein suspending agents may be included, in tablets wherein binders and lubricants may be included, or in a suspension in water or a syrup. Where desirable or necessary, flavoring, preserving, suspending, thickening, or emulsifying agents may be included. Tablets and granules are preferred oral administration forms, and these may be coated.

Parenteral administration, if used, is generally characterized by injection. Injectables can be prepared in conventional forms, either as liquid solutions or suspensions, solid forms suitable for solution or suspension in liquid prior to injection, or as emulsions. A more recently revised approach for parenteral administration involves use of a slow release or sustained release system, such that a constant level of dosage is maintained. See, e.g., U.S. Pat. No. 3,710,795, which is incorporated by reference herein.

For solid compositions, conventional nontoxic solid carriers include, for example, pharmaceutical grades of mannitol, lactose, starch, magnesium stearate, sodium saccharin, talc, cellulose, glucose, sucrose, magnesium carbonate, and the like. Liquid pharmaceutically administrable compositions can, for example, be prepared by dissolving, dispersing, etc. an active compound as described herein and optional pharmaceutical adjuvants in an excipient, such as, for example, water, saline, aqueous dextrose, glycerol, ethanol, and the like, to thereby form a solution or suspension. If desired, the pharmaceutical composition to be administered may also contain minor amounts of nontoxic auxiliary substances such as wetting or emulsifying agents, pH buffering agents and the like, for example, sodium acetate, sorbitan monolaurate, triethanolamine sodium acetate, triethanolamine oleate, etc. Actual methods of preparing such dosage forms are known, or will be apparent, to those skilled in this (84).

The present invention also provides a method for producing single chain antibodies against tumor antigens comprising producing a fusion polypeptide comprising a viral chemokine region and a region comprising a tumor antigen; immunizing animals with an amount of the fusion polypeptide sufficient to produce a humoral immune response to the fusion polypeptide; isolating spleen cells expressing immunoglobulin specific for the fusion polypeptide; isolating the immunoglobulin variable genes from the spleen cells; cloning the immunoglobulin variable genes into an expression vector; expressing the immunoglobulin variable genes in a bacteriophage; infecting E. coli cells with the bacteriophage; isolating bacteriophage from the E. coli cells which express the immunoglobulin variable genes and isolating the immunoglobulin variable gene products for use as single chain antibodies.

The viral chemokine-scFv fusion proteins described herein would be better targets than tumor cells or purified tumor antigen peptides for antibody selection approaches such as phage displayed scFv production. For example, there are two ways to produce specific Fv displayed on the surface of phage: (1) Immunize mice with tumor cells; isolate immunoglobulin variable fragment genes from spleen cells by RT/PCR; clone the genes into bacteriophage in frame with genes coding phage surface proteins (e.g., major coat protein subunits gpVIII or gp III of the filamentous bacteriophage) (93,94); and (2) Construct semisynthetic antibody libraries by PCR as described (95). The specific phage producing scFv are selected by several rounds of binding elution and infection in E. coli, using biotin labeled chemokine-tumor antigen (e.g., Muccore). The biotin enables selection of high affinity scFv-phage through binding to streptavidin conjugated magnetic beads. This approach provides simple, fast and efficient production of specific anti-tumor epitope scFv.

As described herein, the present invention also provides a nucleic acid which encodes a fusion polypeptide of this invention and a vector comprising a nucleic acid which encodes a fusion polypeptide of this invention, either of which can be in a pharmaceutically acceptable carrier. Such nucleic acids and vectors can be used in gene therapy protocols to treat cancer as well as to treat or prevent HIV infection in a subject.

Thus, the present invention further provides a method of treating a cancer in a subject diagnosed with a cancer comprising administering the nucleic acid of this invention to a cell of the subject under conditions whereby the nucleic acid is expressed in the cell, thereby treating the cancer.

A method of treating a B cell tumor in a subject diagnosed with a B cell tumor is also provided, comprising administering the nucleic acid of this invention, encoding a viral chemokine and an antibody or fragment thereof, in a pharmaceutically acceptable carrier, to a cell of the subject, under conditions whereby the nucleic acid is expressed in the cell, thereby treating the B cell tumor.

The methods of this invention comprising administering nucleic acid encoding the fusion protein of this invention to a subject can further comprise the step of administering a nucleic acid encoding an adjuvant such as an immunostimulatory cytokine to the subject, either before, concurrent with or after the administration of the nucleic acid encoding the fusion protein, as described herein.

The nucleic acid can be administered to the cell in a virus, which can be, for example, adenovirus, retrovirus and adeno-associated virus. Alternatively, the nucleic acid of this invention can be administered to the cell in a liposome. The cell of the subject can be either in viva or ex viva. Also, the cell of the subject can be any cell which can take up and express exogenous nucleic acid and produce the fusion polypeptide of this invention. Thus, the fusion polypeptide of this invention can be produced by a cell which secretes it, whereby it binds a viral chemokine receptor and is subsequently processed by an antigen presenting cell and presented to the immune system for elicitation of an immune response. Alternatively, the fusion polypeptide of this invention can be produced in an antigen presenting cell where it is processed directly and presented to the immune system.

If ex vivo methods are employed, cells or tissues can be removed and maintained outside the body according to standard protocols well known in the art. The nucleic acids of this invention can be introduced into the cells via any gene transfer mechanism, such as, for example, virus-mediated gene delivery, calcium phosphate mediated gene delivery, electroporation, microinjection or proteoliposomes. The transduced cells can then be infused (e.g., in a pharmaceutically acceptable carrier) or transplanted back into the subject per standard methods for the cell or tissue type. Standard methods are known for transplantation or infusion of various cells into a subject.

For in vivo methods, the nucleic acid encoding the fusion protein can be administered to the subject in a pharmaceutically acceptable carrier as described herein.

In the methods described herein which include the administration and uptake of exogenous DNA into the cells of a subject (i.e., gene transduction or transfection), the nucleic acids of the present invention can be in the form of naked DNA or the nucleic acids can be in a vector for delivering the nucleic acids to the cells for expression of the nucleic acid to produce the fusion protein of this invention. The vector can be a commercially available preparation, such as an adenovirus vector (Quantum Biotechnologies, Inc. (Laval, Quebec, Canada). Delivery of the nucleic acid or vector to cells can be via a variety of mechanisms. As one example, delivery can be via a liposome, using commercially available liposome preparations such as LIPOFECTIN, LIPOFECTAMINE (GIBCO-BRL, Inc., Gaithersburg, Md.), SUPERFECT (Qiagen, Inc. Hilden, Germany) and TRANSFECTAM (Promega Biotec, Inc., Madison, Wis.), as well as other liposomes developed according to procedures standard in the art. In addition, the nucleic acid or vector of this invention can be delivered in vivo by electroporation, the technology for which is available from Genetronics, Inc. (San Diego, Calif.) as well as by means of a SONOPORATION machine (ImaRx Pharmaceutical Corp., Tucson, Ariz.).

Vector delivery can also be via a viral system, such as a retroviral vector system which can package a recombinant retroviral genome (see e.g., 96,97). The recombinant retrovirus can then be used to infect and thereby deliver to the infected cells nucleic acid encoding the fusion polypeptide. The exact method of introducing the exogenous nucleic acid into mammalian cells is, of course, not limited to the use of retroviral vectors. Other techniques are widely available for this procedure including the use of adenoviral vectors (98), adeno-associated viral (AAV) vectors (99), lentiviral vectors (100), pseudotyped retroviral vectors (101). Physical transduction techniques can also be used, such as liposome delivery and receptor-mediated and other endocytosis mechanisms (see, for example, 102). This invention can be used in conjunction with any of these or other commonly used gene transfer methods.

Various adenoviruses may be used in the compositions and methods described herein. For example, a nucleic acid encoding the fusion protein can be inserted within the genome of adenovirus type 5. Similarly, other types of adenovirus may be used such as type 1, type 2, etc. For an exemplary list of the adenoviruses known to be able to infect human cells and which therefore can be used in the present invention, see Fields, et al. (103). Furthermore, it is contemplated that a recombinant nucleic acid comprising an adenoviral nucleic acid from one type adenovirus can be packaged using capsid proteins from a different type adenovirus.

The adenovirus of the present invention is preferably rendered replication deficient, depending upon the specific application of the compounds and methods described herein. Methods of rendering an adenovirus replication deficient are well known in the art. For example, mutations such as point mutations, deletions, insertions and combinations thereof, can be directed toward a specific adenoviral gene or genes, such as the E1 gene. For a specific example of the generation of a replication deficient adenovirus for use in gene therapy, see WO 94/28938 (Adenovirus Vectors for Gene Therapy Sponsorship) which is incorporated herein in its entirety.

In the present invention, the nucleic acid encoding the fusion protein can be inserted within an adenoviral genome and the fusion protein encoding sequence can be positioned such that an adenovirus promoter is operatively linked to the fusion protein nucleic acid insert such that the adenoviral promoter can then direct transcription of the nucleic acid, or the fusion protein insert may contain its own adenoviral promoter. Similarly, the fusion protein insert may be positioned such that the nucleic acid encoding the fusion protein may use other adenoviral regulatory regions or sites such as splice junctions and polyadenylation signals and/or sites. Alternatively, the nucleic acid encoding the fusion protein may contain a different enhancer/promoter (e.g., CMV or RSV-LTR enhancer/promoter sequences) or other regulatory sequences, such as splice sites and polyadenylation sequences, such that the nucleic acid encoding the fusion protein may contain those sequences necessary for expression of the fusion protein and not partially or totally require these regulatory regions and/or sites of the adenovirus genome. These regulatory sites may also be derived from another source, such as a virus other than adenovirus. For example, a polyadenylation signal from SV40 or BGH may be used rather than an adenovirus, a human, or a murine polyadenylation signal. The fusion protein nucleic acid insert may, alternatively, contain some sequences necessary for expression of the nucleic acid encoding the fusion protein and derive other sequences necessary for the expression of the fusion protein nucleic acid from the adenovirus genome, or even from the host in which the recombinant adenovirus is introduced.

As another example, for administration of nucleic acid encoding the fusion protein to an individual in an AAV vector, the AAV particle can be directly injected intravenously. The AAV has a broad host range, so the vector can be used to transduce any of several cell types, but preferably cells in those organs that are well perfused with blood vessels. To more specifically administer the vector, the AAV particle can be directly injected into a target organ, such as muscle, liver or kidney. Furthermore, the vector can be administered intraarterially, directly into a body cavity, such as intraperitoneally, or directly into the central nervous system (CNS).

An AAV vector can also be administered in gene therapy procedures in various other formulations in which the vector plasmid is administered after incorporation into other delivery systems such as liposomes or systems designed to target cells by receptor-mediated or other endocytosis procedures. The AAV vector can also be incorporated into an adenovirus, retrovirus or other virus which can be used as the delivery vehicle.

As described above, the nucleic acid or vector of the present invention can be administered in vivo in a pharmaceutically acceptable carrier. By “pharmaceutically acceptable” is meant a material that is not biologically or otherwise undesirable, i.e., the material may be administered to a subject, along with the nucleic acid or vector, without causing any undesirable biological effects or interacting in a deleterious manner with any of the other components of the pharmaceutical composition in which it is contained. The carrier would naturally be selected to minimize any degradation of the active ingredient and to minimize any adverse side effects in the subject, as would be well known to one of skill in the art.

The mode of administration of the nucleic acid or vector of the present invention can vary predictably according to the disease being treated and the tissue being targeted. For example, for administration of the nucleic acid or vector in a liposome, catheterization of an artery upstream from the target organ is a preferred mode of delivery, because it avoids significant clearance of the liposome by the lung and liver.

The nucleic acid or vector may be administered orally as described herein for oral administration of the fusion polypeptides of this invention, parenterally (e.g., intravenously), by intramuscular injection, by intraperitoneal injection, transdermally, extracorporeally, topically or the like, although intravenous administration is typically preferred. The exact amount of the nucleic acid or vector required will vary from subject to subject, depending on the species, age, weight and general condition of the subject, the severity of the disorder being treated, the particular nucleic acid or vector used, its mode of administration and the like. Thus, it is not possible to specify an exact amount for every nucleic acid or vector. However, an appropriate amount can be determined by one of ordinary skill in the art using only routine experimentation given the teachings herein (84).

As one example, if the nucleic acid of this invention is delivered to the cells of a subject in an adenovirus vector, the dosage for administration of adenovirus to humans can range from about 10⁷ to 10⁹ plaque forming units (pfu) per injection, but can be as high as 10¹² pfu per injection (104,105). Ideally, a subject will receive a single injection. If additional injections are necessary, they can be repeated at six month intervals for an indefinite period and/or until the efficacy of the treatment has been established.

Parenteral administration of the nucleic acid or vector of the present invention, if used, is generally characterized by injection. Injectables can be prepared in conventional forms, either as liquid solutions or suspensions, solid forms suitable for solution or suspension in liquid prior to injection, or as emulsions. A more recently revised approach for parenteral administration involves use of a slow release or sustained release system such that a constant dosage is maintained. See, e.g., U.S. Pat. No. 3,610,795, which is incorporated by reference herein in its entirety.

The present invention is more particularly described in the following examples which are intended as illustrative only since numerous modifications and variations therein will be apparent to those skilled in the art.

EXAMPLES Example 1 Materials and Methods

Mice and Tumor.

C3H/HeN female mice 6 to 12 weeks of age are obtained from the Animal Production Area of the National Cancer Institute-Frederick Cancer Research and Development Center (NCI-FCRDC, Frederick, Md.). The cell line 38c13 is a carcinogen-induced murine B cell tumor cell line (125). The 38c13 tumor cell secretes and expresses IgM(κ) on the cell surface and is MEM class I positive but class II negative. 38c13 cells from a common frozen stock are passaged in vitro 3 days before use in RPMI 1640 supplemented with 100 U/ml of penicillin and streptomycin, 2×10⁻⁵M 2-mercaptoethanol and heat inactivated 10% fetal bovine serum (BioWhitaker).

Construction of Expression Vectors.

Two types of expression systems are used to produce scFv and scFv fusions. In one system, nucleic acid encoding the fusion protein is expressed in a modified pet11d vector (Stratagene) and purified from inclusion bodies of E. coli. In the second system, the nucleic acid encoding the fusion polypeptide is cloned into a pCMVE/AB (Arya Biragyn) vector under regulatory elements of the early promoter and enhancer of CMV and expressed in the epidermis of mice as a naked DNA vaccine.

Fv fragments are cloned from two different B cell lymphomas, 38C13 and A20, respectively (106,107) by RT/PCR and produced as recombinant fusion peptides with either IP-10, respectively designated as IP10scFv38 and IP10scFv20A, or MCP3scFv38 and MCP3scFv20A. Specifically, lymphoma specific Vh and Vl fragments are cloned by RT/PCR techniques as single chain antibody from total RNA of 38c13 and A20 tumor cells, designated scFv38 and scFv20A respectively, using the following primers.

PRVh-5′: PRV_(H)38-5′: (SEQ ID NO: 4) CTCGAGG TGAAGCTGGTGGAGTCTGGA PRVh-3′: PRV_(H)38-3′: (SEQ ID NO: 5) AGAGGAGACTGTGAGAGTGGTGCCTT PRVl-5′: PRV_(L)38-5′: (SEQ ID NO: 6) GACATCCAGATGACACAGTCTCCA PRVl-31: PRV_(L)38-3′: (SEQ ID NO: 7) GGATCCTTTTATTTCCAGCTTGGTCCCCCCTCCGAA PRV_(H)20A-5′: (SEQ ID NO: 8) CCATGGTCCAAC TGCAGCAGTCAGGGCCTGAC PRV_(H)20A-3′: (SEQ ID NO: 9) TGAGGAGACTGTGAGTTCGGTACCTT GGCC PRV_(L)20A-5′: (SEQ ID NO: 10) GATGTTGTGATGACGCAGACTCCACTC PRV_(L)20A-3′: (SEQ ID NO: 11) GGATCCTTTGACTTCCAGCTTTGTGCCTCCA

The resulting scFv contained a (GIy₄Ser)₃ linker and is cloned into the expression vector pET11d, which is modified to fuse in frame with c-myc and the His tag peptide sequences, followed by an amber stop codon. The resulting scFv contains a 17 a.a. residue linker, GGGGSGGGGSGGGGSGS (Gly₄Ser)₃GlySer (SEQ ID NO:12) (108).

Constructs for the nDNA vaccination are fused in frame to a leader sequence of vMIPI in pCMVE/AB to enable secretion. The carboxy-terminus of scFv is fused in frame with the tag sequence encoding c-myc peptide and six His residues, respectively: GGA TCC GCA GAA GAA CAG AAA CTG ATC TCA GAA GAG GAT CTG GCC CAC CAC CAT CAC CAT CAC TAA CCCGGG (SEQ ID NO:13). Genes for the mature sequence of viral chemokines vMIPI, vMIPII, and vMIPII are cloned by RT/PCR technique from cell lines infected with HHV-8 as would be known in the art, and fused in frame with sFv utilizing suitable primers to form vMIPIsFv38, vMIPIIsFv38 and vMIPIIIsFv38.

VMIPII, vMIPII, or vMIPIII or control viral epitope (PreS2 and DomA) fusions are made by fusing them to amino-terminus of scPv through a short spacer sequence: 5′ GAA TTC AAC GAC GCT CAG GCG CCG AAG AGT CTC GAG 3′ (SEQ ID NO:14), encoding the amino acid sequence: EFNDQAPKSLE (SEQ ID NO:15). Two unique restriction endonuclease sites are introduced at the ends of the space to facilitate cloning: EcoRI at the 5′ end (underlined) and XhoI at the 3′ end (underlined). All constructs are verified by DNA dideoxy-sequencing method, using T7 SEQUENASE kit (Amersham).

vMIPI, vMIPII, and vMIPIII chemokines are cloned into the scFv38 expression vector through NcoI and XhoI restriction sites. The resulting fusion nucleic acid contains the viralchemokine gene ligated to the 5′-end of the scFv38 gene and separated with a short spacer sequence, as described above.

Bacterial Expression and scFv Purification.

The recombinant proteins are expressed in BL21(DE3) cells (InVitrogen) as inclusion bodies after 8 hours of induction in Super-Broth with 0.8 mM IPTG in the presence of 150 μg/ml carbenicillin and 50 μg/ml ampicillin at 30° C. vMIPI-scFv38 and vMIPII-scFv38 are purified from the inclusion bodies with a modified method (110). Briefly, inclusion bodies, denatured in 6M GuHCl, 100 mM NaH₂PO₄, 10 mM Tris-HCl, pH 8.0, are reduced in 0.3M DTE and refolded at a concentration of 80 μg/ml in the refolding solution (Tris-HCl, pH 8.0, 0.5M arginine-HCL, 4 mM GSSG and 2 mM EDTA) for 72 hours at 10° C. The refolded solution is dialyzed in 100 mM Urea and 20 mM tris-HCl, pH 7.4 and the recombinant protein is purified by binding to heparin-sepharose resins (Pharmacia, Biotech, Uppsala, Sweden). The integrity and purity of the recombinant protein is tested by PAGE gel electrophoresis in reducing conditions and by Western blot hybridization with mAb 9E10. The purification yields 2-20 mg/l of the soluble protein with greater than 90% purity.

Results

Purified fusion polypeptide is tested for the ability to inhibit binding of native IgM 38c13 (Id38), as compared to positive sera from mice immunized with Id38−KLH. ELISA plates are coated with 10 μg/ml Id38, then wells are incubated with anti-Id38 positive sera (1:500) and titrated amounts of scFv. Id38 (10 μg/ml) and either vMIPIscFv20 or vMIPIIscFv20 (vMIPI, vMIPII or vMIPIII fused to an irrelevant scFv) are used as positive and negative control samples, respectively.

Recombinant fusion proteins purified from E. coli are characterized for proper idiotype folding by their ability to inhibit 38c13 IgM binding to a monoclonal (SIC5 mAb) or polyclonal anti-idiotypic sera, in order to determine if vMIPI, vMIPII, or vMIPIII vMIPIII fusions interfere with the proper conformation of scFv38. Next, receptor binding experiments are used to determine whether either vMIPI, vMIPII, or vMIPIII fused scFv, but not control viral epitope DomA fused scFv38 (DomAsav38), bind to their chemokine receptors. Accordingly, vMIPIsFv38, vMIPIIsFv38, and vMIPIIIsFv38 are each tested for their ability to bind to CCR5 and CXCR4 transfected cell lines as known in the art. vMIPIIsFv38 does bind to CCR5 and CXCR4 transfected cell lines, as evidenced by the ability of vMIPIIsFv38 to displace labeled MIP1.

Furthermore, vMIPIsFv38, vMIPIIsFv38, and vMIPIIisFv38 are tested for their ability to induce chemotaxis of THP-1 cells. As expected, vMIPIIsFv38 does not induce chemotaxis, while vMIPIsFv38 does retain chemotaxis activity.

In Vivo Immunization and Tumor Protection.

To test the ability of vMIPIsFv38, vMIPIIsFv38, and vMIPIIIsFv38 to render self tumor antigen, sFv38, immunogenic when immunized as genetic vaccine in mice, ten mice per group are gene-gun immunized with plasmid encoding fusions with the viral chemokine fusions pvMIPIsFv38, pvMIPIIsFv38, and pvMIPIIIsFv38 in order to demonstrate whether these fusions can target APC in vitro. As a control, mice are immunized with the similar DNA constructs but encoding mutated chemokine fusions pvMIPIDsFv38, pvMIPIIDsFv38, and pvMIPIIIDsFv38. The viral chemokines vMIPI and vMIPII induce significant anti-idiotype specific antibodies compared to the prototype Ig38-KLH protein vaccine. These results are in distinct contrast with the lack of any anti-idiotypic antibody response after immunization with fusions with mutated chemokines. Thus, the non-immunogenic sFv is rendered immunogenic by viral chemokines, and the response correlates with the ability to induce chemotaxis of immature DC and other APC.

Groups of ten mice immunized with viral chemokine or control plasmids are challenged with 20-fold lethal dose of tumor two weeks after the last of three serial immunizations. Mice immunized with viral chemokine mutants pvMIPIDsFv38 and pvMIPIIDsFv38, similarly to mice immunized with corresponding active chemokines fused with sFvA20 from irrelevant lymphoma A20 sFv or PBS, do not survive. In contrast, pvMIPIsFv38 or pvMIPIIsFv38 immunized mice demonstrate statistically significant survival. The survival closely correlates with the presence of functionally intact or active viral chemokines which can act on immature DC or other APC via differentially expressing their receptors. Although Gen-gun bombarded DNA does target a variety of skin cells including skin APC and LC, it is not sufficient to render self-tumor antigen (sFv) immunogenic. Instead, physical linkage of sFv with viral chemokine moieties is required. No positive humoral response or survival is detected in mice immunized with DNA plasmids expressing free unlinked viral chemokine and sFv38.

Thus, the animal experiments clearly correlate with functional data from in vitro studies. Id-specific responses and tumor immunity is detected only when the viral chemokine moiety in the fusion retains the functional properties of the respective viral chemokine, while no immunity is observed when the viral chemokine is replaced with a mutant, functionally inactive chemokine. Furthermore, induction of chemotaxis to the site of vaccine injection or production is not sufficient to generate, as demonstrated by the lack of humoral and anti-tumor immunity in mice immunized with viral chemokine alone or with either a mixture of free, unlinked viral chemokine and sFv or viral chemokine fused with an irrelevant sFv.

Example 2

Recent experiments also demonstrate that vMIP-II elicits antigen specific responses against human breast cancer Muc-1 antigen and env protein of HIV-1.

Six- to nine-week old female C3H/HeN mice are immunized intraperitoneally (i.p.) with 100 to 200 μg of the soluble protein in PBS and control immunogen Id38-KLH two times at two week intervals or are shaved and immunized by Accell gene delivery device (Agracetus, Inc., Middleton, WN) with 1 μg gold particles carrying 1-3 μg plasmid DNA. Sera are collected by orbital bleeding two weeks after each vaccination. Serum anti-idiotypic (anti-Id) antibody levels are tested as described (111) over microliter plates coated with 10 μg/ml native IgM 38c13. Two weeks after the last immunization, mice are inoculated with 2000 38c13 tumor cells i.p. Survival is determined, and significance with the respect to time to death, is assessed using BMDP IL software (BMDP statistical software, Los Angeles). Mice are observed daily for any signs of toxicity and date of death and animals surviving >80 days after tumor challenge are killed and reported as long-term survivors.

Mice are immunized either with a plasmid coding for a vMIPIsFv38 fusion, a vMIPIIsFv38 fusion, a vMIPIIIsFv38 fusion, or a mixture of DNA constructs expressing unlinked scFv38 and vMIPIscFv20A (scFv38D+vMIPIscfv20AD).

Ten mice per group are immunized with two types of scFv38 fused to vMIPI, vMIPII or vMIPIII, differing only in orientation of variable genes in scFv. Control mice receive IgM-KLH (Id38-KM) and vMIP fusion to A20 lymphoma scFv (IP10scFv20A). Ten mice per group are immunized i.d. with plasmid coding either for viral chemokine fusion vaccine (vMIPIscFv38D, vMIPIIscFv38D, or MIPIIIscFv38D), or free scFv (scFv38D), or viral epitope preS2 fused scFv (PreS2scFv38D).

Effector CD8⁺ and CD4⁺ cells are depleted two weeks after the last immunization with three i.p. injections of 400 μg α-CD8 mAb 53.6.72, or α-CD4 mAb GK1.5 (both ammonium sulfate purified ascites, Biological Resource Branch, NCI-FCRDC) (32,34), or control rat IgG (Sigma). Control mice are immunized with plasmid expressing vMIPI, vMIPII, or vMIPIII fused to A20 scFv (MCP3scFv20AD).

Ten Balb/C mice per group are immunized i.p. twice with 100 μg of vMIPI, vMIPII, or vMIPIII fused with scFv20A protein in PBS (vMIPIscFv20A and vMIPIIscFv20A, respectively) and challenged i.p. with 10⁵ A20 tumor cells. To determine the role of free versus linked chemokine, vMIPIscFv20A is co-injected with vMIPII fused to an irrelevant scFv38 (vMIPIscFv20A+vMIPIIscFv38). Control mice are immunized with A20 IgM-KLH (Id20A-KLH).

Immunoassays and Serum Anti-Idiotypic Antibody.

The assessments for correct folding of purified scFv38 and fusion scFv38 are determined by ELISA with mAbs and by inhibition assay with Id38−KLH sera (immunized with native IgM 38c13 conjugated to KLH). Briefly, microtiter plates (Nunc, Naperville, Ill.) are coated overnight at 4° C. with 10 μg/ml anti-c-myc mAb 9E10 in carbonate buffer (50 mM NaHCO₃, pH 9.0). The wells are blocked with 5% nonfat dry milk in PBS for 30 min. Plates are washed in 0.05% Triton X-100 in PBS, and serially diluted scFv (starting from 10 μg/ml in 50 μl % BSA/PBS) is applied, after which plates are incubated 40 min at room temperature. After washing, the wells are incubated with 50 μl of 1:300 diluted biotinylated anti-Id38 mAb in 2% BSA/PBS for 30 min at room temperature. Wells are washed and incubated with streptavidin-HRP conjugate (1:5000) in 2% BSA/PBS for 30 min at room temperature. Then, wells are washed and incubated with ABTS peroxidase substrate (KPL, Gaithersburg, Md.) and the absorbance at 405 nm is measured.

Inhibition assays are performed as described above, except plates are coated with 10 μg/ml of native IgM 38c13, then wells are incubated for 30 min at room temperature with a 1:2 dilution of positive Id38−KLH sera mixed with serially diluted purified scFv proteins starting from 50 μg/ml in 2% BSA/PBS. The bound antibodies from the sera are assayed by incubating wells for 30 min at room temperature with anti-mouse IgG-HRP mAb (Jackson).

Serum anti-idiotypic (anti-Id) antibody levels are tested as described (37). Briefly, mouse serum is serially diluted over microtiter plates coated with 10 μg/ml native IgM 38c13. Binding of antibodies in the serum to 38c13 IgM is detected by goat anti-mouse IgG-HRP. Serum anti-Id antibody levels are quantitated by comparing sera titration curves with a standard curve obtained with a known concentration of a mixture of purified monoclonal anti-Id antibodies. Antibody levels are expressed in g/ml of serum for individual mice. In each ELISA, sera obtained from mice immunized with control IgM-KLH are included as negative controls. Such sera never showed any titration binding activity on Id-38c13.

In Vitro and In Vivo Chemotaxis Assays.

Single cell suspensions are prepared from spleens of untreated C3H/HeJ mice. Murine T cell enrichment columns (R&D System, Minneapolis, Minn.) are then used to prepare a purified murine T cell population via high-affinity negative selection according to the manufacturer's instructions. The isolation procedure typically yields over 89% CD3⁺ T cells, as determined by FACS analysis. T cell migration in vitro is assessed by 48-well microchemotaxis chamber technique. Briefly, a 26 μl aliquot of the recombinant scFv fusion protein serially diluted in the chemotaxis medium (RPMI 1640, 1% BSA, 25 mM HEPES) is placed in the lower compartment and 50 μl of cell suspension (5×10⁶ cells/ml) is placed in the upper compartment of the chamber. The two compartments are separated by a polycarbonate filter (5 μm pore size; Neuroprobe, Cabin John, Md.) coated with 10 μg/ml of fibronectin (Sigma, St. Luis, Mo.) and incubated overnight at 4° C. or for 2 hours at 37° C. The chemotaxis assay is performed at 37° C. for 2 hours. Then the filter is removed, fixed and stained with Diff-Quik (Harlew, Gibbstown, N.J.), The number of migrated cells in three high power fields (400×) is counted by light microscopy after coding the samples. The results are expressed as the mean±SE value of the migration in triplicate samples.

T cell migration in vitro is assessed by the 48-well micro chemotaxis chamber technique as described (112). Single cell suspensions are prepared from spleens of untreated C3H/HeJ mice. Murine T cell enrichment columns (R&D System, Minneapolis, Minn.) are then used to prepare a purified murine T cell population via high-affinity negative selection according to the manufacturer's instruction. The isolation procedure typically yields over 89% CD3⁺ T cells, as determined by FACS analysis.

In order to test in vivo effects on cell accumulation, C3H/HeN mice are injected s.c. with a single 10 μg dose of scFv fusion proteins. Portions of the skin from the site of injection are removed 72 hours after the injection, fixed in 10% neutral buffered formalin, embedded in paraffin, sectioned at 5 μm and stained with hematoxylin and eosin (H&E). Slides are evaluated microscopically without knowledge of the experimental treatment.

In Vivo Cellular Infiltration into Murine Skin.

The numbers of PMN and mononuclear (MN) cells infiltrated into murine skin are graded as following:—, no significant lesion; 1, mild; 2, moderate; 3 severe; F, focal; MF, multi focal. Mice are injected with 10 μg of vMIPIscFv38, vMIPIIscFv38, vMIPIIscFv38, preS2scFv38 (N18), or PBS, subcutaneously. After 72 h, the injection site is excised and examined histologically on coded slides to determine the extent of infiltration. The amount of endotoxin injected with samples is 0.5-1 units.

Chemokine Binding Assay and Confocal Microscopy.

Chemokine binding assays are performed using laser confocal microscopy (113). Purified T cells or spleen cells from C3H mice are used at ˜1×10⁶ per ml and are incubated with 100 nM viral chemokine-scFv (vMIPIscFv38, vMIPIIscFv38, or vMIPIIscFv38), or control viral epitope-scFv for 1 hour at 37° C. For the ligand competition assay, 100 nM chemokine-scFv is incubated with 500 nM of the corresponding chemokine (IP-10 or MCP-3). Samples are washed 2× in PBS and fixed in suspension with 2% paraformaldehyde.

The samples are incubated at RT for 15 min. Slides containing the samples are incubated in 9E10 anti c-myc mAb primary antibody at a 1:50 dilution in wash buffer (0.25% gelatin, 0.15% saponin, 1% goat serum in PBS). Slides are then incubated with goat anti-mouse IgG F(ab′)2-FITC (Boehringer-Mannheim) at a 1:50 dilution for 30 min at RT in a humidified chamber. Slides are washed 3×5 min in 0.25% gelatin, 0.15% saponin in TBS. Slides are then incubated for 10 min in a 1:100 dilution of DAPI, washed 2× briefly in TBS, then 1× briefly in dH₂O, air-dried and mounted using aqueous mounting medium appropriate for immunofluorescence (Gel/Mount, Biomeda).

The Traditional Approach to Enhance Immunogenicity by Cross Linking to KLH is not Effective.

Several different approaches are used for the production of single chain antibody fragments from 38c13 cells (scFv38) in E. coli. Yield of scFv38 differ significantly depending on the method used. Production of scFv38 through a secretory path using a PelB leader sequence as a native protein is least efficient. The problem is solved when scFv38 is produced as insoluble “inclusion” bodies, which yield about 2-8 mg of refolded scFv per liter of the batch culture with greater than 90% purity. Folding properties of the produced scFv38 are monitored by either (i) inhibition assay with native Id38; or (ii) modified ELISA assay where scFv38 is captured through an anti-c-myc tag and detected with the biotinylated monoclonal anti-Id38 antibody (anti-Id38 mAb does not recognize linear or incorrectly folded epitope). These experiments demonstrate that scFv38, but not irrelevant scFv20A, specifically binds to anti-Id38c mAb and inhibits binding of the native Id38c to anti-Id38c mAb, 50% binding inhibition by 10-15 fold excess of scFv38. In addition, positive sera from Id38c-KLH immunized mice specifically recognizes purified scFv38. These data indicate that purified scFv38 is folded correctly and imitates the idiotype of the native antibody (Id38c) of B cell lymphoma 38c13.

Immunization experiments showed that scFv38, similarly to the native Id38c IgM, is a poor immunogen. Attempts were made to convert scFv38 into a potent immunogen by chemical cross linking with KLH, in analogy to the native Id38c. However, in contrast to Id38−KLH, i.p. immunizations of syngeneic mice with 100 μg of scFv38−KLH did not elicit any anti-Id38c specific antibody response. This inability to induce anti-Id38 response correlates with the loss of ability to affect binding of anti-Id38 mAb (SIC5) to Id38c by samples containing scFv38−KLH, while a control sample of an equimolar mixture of non-cross linked scFv38 and KLH (scFv38+KLH) inhibited anti-Id38/Id38c binding similarly to pure scFv38. These data indicate that a fragile Id conformation of scFv38 is removed by KLH cross linking and that this traditional approach is not applicable for the enhancement of immunogenicity of scFv38.

Design and Production of Chemokine Fused scFv38.

Viral MIPI, MIPII and vMIPIII are subcloned from cell lines infected with HHV-8 by RT/PCR using specific primers as described herein and inserted in frame in front of the scFv38 DNA sequence. The resulting fusion gene is designated as vMIPIscFv38, vMIPIIscFv38, and vMIPIIIscFv38, respectively. In order to evaluate input of the immunoglobulin V chain specific orientation, two variants of fusion chemokine-scFv genes are designed, one containing a V_(H)-V_(L) and one containing a V_(L)-V_(H) sequence, respectively designated as scFv38MH and scFv38(INV)MH.

All fusion proteins used in these experiments are purified from inclusion bodies of E. coli, solubilized and refolded as described herein. A spacer sequence, as described herein, is introduced into the chemokine fusion proteins and correct folding is tested for each recombinant protein.

The ability of vMIPIscFv38, vMIPIIscFv38 and vMIPIIIscFv38 proteins to induce chemotaxis in vivo in C3H/HeN mice is also tested. Mice are s.c. injected once with 10 μg of the fusion protein and after 72 hours, the skin around the site of injection is removed and analyzed as described herein.

Production of Fusion Polypeptides Comprising a Human Chemokine and a Human Tumor Antigen or HIV Antigen.

To produce the fusion polypeptides of the present invention which comprise a viral chemokine region and a human tumor antigen region or HIV antigen region, the following procedures are carried out: Tumor or viral antigen is cloned by PCR or RT/PCR from DNA or RNA of biopsy cells of a patient, using specific primer. The primers are made using standard methods for selecting and synthesizing primer sequences from analysis of known sequences of the genes of interest (e.g., from GenBank, Kabat Ig sequence database and other available genetic databases, as are known in the art). For example, lymphoma or myeloma-specific scFv is cloned by RT/PCR from the nucleic acid from a patient's lymphoma or myeloma biopsy cells or from nucleic acid from hybridoma cells expressing the patient's immunoglobulin. Several sets of primers are used to clone human variable (V) genes based on GenBank and Kabat IG sequence data. As in cloning murine scFv, human tumor V fragments are cloned and sequenced using a family-specific primer or primer mixture for leader and constant region sequences. Next, scFv is constructed using primers based on the sequence of each V gene cloned. These primers can have specific restriction endonuclease sites to facilitate routine cloning, or scFv is made by overlapping PCR, according to methods well known in the art. The vector expressing the fusion polypeptide can contain several unique restriction endonuclease sites (e.g., XhoI, BamHI) between the 3′ end of the spacer sequence and the 5′ end of the c-myc and six His tag sequences, or the 5′ end of the polyA transcription terminator region (if a SmaI site is used), thus enabling routine cloning of any scFv, tumor antigen or viral antigen.

As described herein, nucleic acid encoding the viral chemokine-tumor antigen fusion polypeptides of this invention is expressed in yeast (e.g., Saccharomyces cerevisiae; Pichia pastoris, etc.) or in mammalian cell culture according to methods standard in the art. The proteins produced in these systems are affinity purified with anti-c-myc antibodies (e.g., 9E10; M5546, Sigma) or anti-poly-His antibodies (e.g., H1029, Sigma). Alternatively, immobilized metal chelate affinity chromatography (Ni-NTA resin, Qiagen) is used for purification of soluble or refolded fusion polypeptides.

Administration of Fusion Polypeptides to Human Subjects.

Immunity and suppression of tumor growth in a human subject. To elicit a tumor cell growth-inhibiting response in a human subject, a fusion polypeptide comprising a viral chemokine and a tumor antigen which is present in the human subject is administered to the subject subcutaneously in a dose ranging from 1 to 500 μg of the fusion polypeptide once weekly for about eight weeks or once monthly for about six months. Within the first month following the initial immunization, blood samples can be taken from the subject and analyzed to determine the effects of administration of the fusion polypeptide. Particularly, the presence in the subject's serum, of antibodies reactive with the tumor antigen in the fusion protein can be determined by ELISA, Western blotting or radioimmunoprecipitation, or other methods for detecting the formation of antigen/antibody complexes as would be standard practice for one of ordinary skill in the art of immunology. Also, a cellular immune response to the tumor antigen in the fusion polypeptide can be detected by peripheral blood lymphocyte (PBL) proliferation assays, PBL cytotoxicity assays, cytokine measurements, or other methods for detecting delayed type hypersensitivity and cellular immune response, as would be standard practice for one of ordinary skill in the art of immunology. Additionally, the kinetics of tumor growth and inhibition of tumor cell growth can be determined by monitoring the subject's clinical response, through physical examination, tumor measurement, x-ray analysis and biopsy. The exact dosage can be determined for a given subject by following the teachings as set forth herein, as would be standard practice for one of ordinary skill in the art of vaccine development.

Example 3

This example demonstrates that antigens elicit effective immunity when they are targeted to APC, particularly iDC, via chemokine receptors as fusions with proinflammatory chemokines factors. Moreover, this example demonstrates that proinflammatory factors such as murine β-defensins induce chemotaxis of immature, but not mature, DC and, thus, can serve effectively as an carrier for targeting antigens to APC. Non-immunogenic tumor antigens or xenogeneic HIV gp120 antigen were rendered effectively immunogenic when immunized as fusion with murine β-defensin 2. This example also demonstrates the use of xenogeneic human and viral chemokines such as Kaposi's sarcoma virus derived chemokine analogues of human MIP-1s, designated vMIP1 and vMIP2 (Nicholas, J., V. R. Ruvolo, W. H. Burns, G. Sandford, X. Wan, D. Ciufo, S. B. Hendrickson, H. G. Guo, G. S. Hayward, and M. S. Reitz. 1997. Kaposi's sarcoma-associated human herpesvirus-8 encodes homologues of macrophage inflammatory protein-1 and interleukin-6. Nat. Med. 3:(3)287-292), which bind multiple receptors on murine cells and which might circumvent the potential development of autoimmunity against host chemokine carriers (Luster, A. D. 1998. Chemokines-chemotactic cytokines that mediate inflammation. N. Engl. J. Med. 338:(7)436-445; Pelchen-Matthews, A., N. Signoret, P. J. Klasse, A. Fraile-Ramos, and M. Marsh. 1999. Chemokine receptor trafficking and viral replication. Immunol Rev. 168:3349:33-49). In addition, using a pair of viral chemokines that bind to CCR8, the agonist vMIP1 (Endres, M. J., C. G. Garlisi, H. Xiao, L. Shan, and J. A. Hedrick. 1999. The Kaposi's sarcoma-related herpesvirus (KSHV)-encoded chemokine vMIP-I is a specific agonist for the CC chemokine receptor (CCR)8. J. Exp. Med. 189:(12)1993-1998) and antagonist MC148, expressed by Molluscum contagiosum virus (MCV) (Luttichau, H. R., J. Stine, T. P. Boesen, A. H. Johnsen, D. Chantry, J. Gerstoft, and T. W. Schwartz. 2000. A highly selective CC chemokine receptor (CCR)8 antagonist encoded by the poxvirus molluscum contagiosum. J. Exp. Med. 191:(1)171-180), this example demonstrates that antigen targeting alone in the absence of chemotaxis is sufficient for induction of immunity.

Methods

Fusion Gene Cloning and Plasmid Constructions.

Cloning strategy for lymphoma specific V_(H) and V_(L) fragments from 38C13 (Bergmanm Y. and J. Haimovich. 1977. Characterization of a carcinogen-induced murine B lymphocyte cell line of C3H/eb origin. J. Immunol. 7:413417) and A20 (Kim, K J., L. C. Kanellopoulos, R. M. Merwin, D. H. Sachs, and R. Asofsky. 1979. Establishment and characterization of BALB/c lymphoma lines with B cell properties. J. Immunol. 122:(2)549-554) cells as sFv38 and sFv20, respectively, has been reported elsewhere (Biragyn, A., K. Tani, M. C. Grimm, S. D. Weeks, and L. W. Kwak. 1999. Genetic fusion of chemokines to a self tumor antigen induces protective, T-cell dependent antitumor immunity. Nature Biotechnology 17:253-258). Genes for mature human and murine chemokines and defensins were cloned in frame to the 5′-end of sFv by RT/PCR from total RNA using specific primers as described previously (Biragyn, A., K. Tani, M. C. Grimm, S. D. Weeks, and L. W. Kwak. 1999. Genetic fusion of chemokines to a self tumor antigen induces protective, T-cell dependent antitumor immunity. Nature Biotechnology 17:253-258). For example: genes for human MDC (GeneBank # HSU83171) and SDF-1β (GeneBank # HSU16752) were cloned from LPS 10 ng/ml treated human monocytes using respectively pairs of primers PRhMDC-5′ (CTCTAGACACCATGOCTCGCCTACAGACTGCACT; SEQ ID NO:16) and PRhMDC-3′ (TGAATTGITGGCTCAGCTTATTGAGAATCA; SEQ ID NO:17); and PRhSDF1β-5′ (CTCTAGACACCATGAACGCCAAGGTCGTGGTCGTGCTG; SEQ ID NO:18) and PRhSDF1β-3′(TGAATTCCATCTTGAACCTCTTGTTTAAAGCTTT; SEQ ID NO:19). Murine β-defensin 2 (GeneBank # AJ011800) and (3-defensin 3 (GeneBank # AF092929) genes were cloned from LPS (10 ng) Balb/c mouse skin using pairs of primers, respectively PRmDF2β-5′ (ACCATGGAACTTGACCACTGCCACACC; SEQ ID NO:20) and PRmDF2β-3′ (TGAATTCAAGATCTTTCATGTACTTGCAACAGGGGTTGTT; SEQ ID NO:21) and PRmDF3β-5′ (ACCATGGAAAAAATCAACAATCAGTAAGTTGTITGAGG; SEQ ID NO:22) and PRmDF3β-3′ (CTCGAGCTAGAATTCTTTTCTCTGCAGCATTTGAGGAAA; SEQ ID NO:23). Similarly, murine (3-pro-defensin 2 gene was cloned for eukaryotic expression using PrproDF2βL-5′ (AAAGCTTCCACCATGAGGACTCTCTGCTCT; SEQ ID NO:24) and PRmDF2β-3′, which contained native secretion signal sequence. For bacterial expression, the signal sequence was removed using PRmDF2β-5′ (ACCATGGCTGTTGGAAGTAAAAAGTATTGGA; SEQ ID NO:25) and PRmDF2β-3′. Viral chemokine genes vMIP-I (GeneBank # KSU74585) and vMIP-II (GeneBank # KSU67775) were cloned from BCBL-1 lymphoma cell line infected with HHV-8 (NIH AIDS Research & Ref. Reag. Program), using pairs of primers, respectively PRvMIP1L-5′ (TAAGCTECCACCATGGCCCCCGTCCACGTTTTATGCT; SEQ ID NO:26) and PRvMIP1-3′ (TGAATTCAGCTATGGCAGGCAGCCGCTCATCAGCTOCCT; SEQ ID NO:27) and PRvMIP1IL-5′ (TAAGCTTCACCATGGACACCAAGGGCATCCTGCTCGT; SEQ ID NO:28) and PRvMIP1I-3′ (TGAATTCGCGAGCAGTGACTGGTAATTGCTGCAT; SEQ ID NO:29). Mature sequences of vMIP-I and vMIP-II for expression in bacterial system were cloned using the following pairs of primers: PRvMIP1M-5′(ACCATGGCGGGGTCACTCGTGTCGTACA; SEQ ID NO:30) and PRvMIP1-3′ and PRvMIP2M-5′ (ACCATGGGAGCGTCCTGGCATAGA; SEQ ID NO:31) and PRvMIP1I-3′. MC148 chemokine gene (GeneBank # U96749) was cloned from plasmid DNA containing a portion of Moluscum contagiosum virus type 1 genome (Damon, L, P. M. Murphy, and B. Moss. 1998. Broad spectrum chemokine antagonistic activity of a human poxvirus chemokine homolog. Proc. Natl Acad. Sci. U.S.A. 95:(11)6403-6407) using pairs of primers PRMC148L-5′ (AAAGCTAGCACCATGAGGGGCGGAGACGTCTTC; SEQ ID NO:32) and PRMC148-3′ (AGAATTCCAGAGACTCGCACCCOGACCATAT; SEQ ID NO:33) and PRMC148M-5′ (ACCATGGCACTCGCGAGACGGAAATGTTGTTTGAAT; SEQ ID NO:34) and PRMC148-3′, respectively for eukaryotic and bacterial expression. The carboxy-terminus of sFv was fused in frame with a tag sequence coding c-myc peptide AEEQKLLSEEDLA (SEQ ID NO:35) and six His, respectively. Chemokine and defensins have been fused with sFv through a spacer sequence NDAQAPKS (SEQ ID NO:36). To generate constructs encoding mutant chemokines, the first Cys residue was replaced to Ser for all chemokines, except for hMCP-3 and hMDC where the amino-terminus up to the second Cys residue were truncated. Bacterial expression vectors contained only genes encoding mature peptide genes, while constructs for DNA vaccination were fused in frame to a leader sequence of IP-10 in pCMVE/AB, except for constructs designed for pMDCsFv38 and pSDF1βsFv38 plasmids, which contained their native signal sequences. All constructs were verified by DNA dideoxy-sequencing method, using T7 sequenase kit (Amersham, USA) and purified using Qiagen plasmid purification kit (Qiagen, Valencia, Calif.).

For the second model, gp120 gene was cloned from the plasmid DNA containing portion of HIV-1 (isolate 89.6) in frame with IP-10 secretion signal sequence (pgp120) using primers PRM89.6ENV-5′ (AAAGTCGACAAAGAAAAAACGTGG GTCACAATCT; SEQ ID NO:37) and PR89.6ENV-3′ (ATTCCCGGGTTATITTTCTCTITGCACTGTTCTTCTC; SEQ ID NO:38). Similarly, gp120 was fused in frame with coding sequences from murine β-defensin 2, hMDC and hMCP3 to generate DNA constructs pmDF2βgp120, phMDCgp120, phMCP3gp120, respectively.

Recombinant fusion proteins purified as inclusion bodies after 8 hours of induction in Super-Broth (Digene Diagnostics, Inc., Beltsville, Md.) with 0.8 mM IPTG in the presence of 150 μg/ml carbenicillin and 50 μg/ml ampicillin at 30° C., and refolded according to Buchner, et al (Buchner, J., L Pastan, and U. Brinkmann. 1992. A method for increasing the yield of properly folded recombinant fusion proteins: single-chain immunotoxins from renaturation of bacterial inclusion bodies. Anal. Biochem. 205:(2)263-270) with modifications (Biragyn, A., K. Tani, M. C. Grimm, S. D. Weeks, and L. W. Kwak. 1999. Genetic fusion of chemokines to a self tumor antigen induces protective, T-cell dependent antitumor immunity. Nature Biotechnology 17:253-258) from BL21(DE3) cells (Invitrogen, Milford, Mass.). The refolded fusion proteins were purified by heparin-sepharose chromatography (Pharmacia Biotech, Uppsala, Sweden). The integrity and purity of recombinant proteins were tested by PAGE under reducing conditions and by western blot hybridization with 9E10 anti-c-myc mAb (Sigma). Purification usually yielded soluble protein with greater than 90% purity. Correct folding of purified sFv38 proteins were determined by the ability to bind to anti-idiotype mAb S1C5 by ELISA (Biragyn, A., K. Tani, M. C. Grimm, S. D. Weeks, and L. W. Kwak, 1999. Genetic fusion of chemokines to a self tumor antigen induces protective, T-cell dependent antitumor immunity. Nature Biotechnology 17:253-258). Briefly, serially diluted sFv were added to microliter plates coated with 10 μg/ml anti-c-myc mAb 9E10. After washing, plates were incubated with a 1:300 diluting of biotinylated S1C5. Plates were washed, incubated with streptavidin-HRP (1:5000, Jackson Immuno research Lab., Inc., Bar harbor, ME) and developed with ABTS peroxidase substrate (KPL, Gaithersburg, Md.).

Isolation of Murine Bone Marrow Derived Dendritic Cells.

Murine bone marrow derived DC were isolated as described elsewhere (Fields, R. C., Osterholzer, J. A. Fuller, E. K. Thomas, P. J. Geraghty, and J. J. Mule. 1998. Comparative analysis of murine dendritic cells derived from spleen and bone marrow. J. Immunother. 21:(5)323-339). Briefly, bone marrow was collected from tibias and femurs of 4 to 6 months old BALB/c mice by flushing with PBS using a 10 mL syringe with a 27 gauge needle. Erytrocytes were lysed by treatment with ACK lysis buffer (BioWhittaker, Walkersville, Md.). Cells expressing CD8, CD4, B220 and I-A^(b) were depleted using a mixture of mAbs and rabbit complement. The mAbs were TIB-146 (anti-B220), 150 (anti-CD8), TIB-207 (anti-CD4), TIB-229 (anti-1-A^(b)) obtained from ATCC. Cells were then resuspended with DC medium (RPMI 1640 containing 5% heat inactivated fetal bovine serum, 1% penicillin streptomycin, 1% L-glutamine and 5×10⁻⁵ 2-ME) supplemented with 10 ng/mL recombinant murine IL-4 and 10 ng/mL recombinant murine GM-CSF (Peprotech) and cultured in 6 well plates (7×10⁵ cells/mL, 5 ml On day two, 200 μl DC medium containing 10 ng/mL of both IL-4 and GM-CSF were added to each well. Then, at day four, 5 μl of DC medium containing cytokines were added to each well after non-adherant cells were removed, and cells were cultured for additional 4 days. Cells were harvested on day 4 and day 7 and used in subsequent experiments.

In Vitro Chemotaxis Assay:

The chemotactic migration of murine dendritic cells was assessed using a 48-well microchemotaxis chamber technique as previously described (Falk, W., R. H. J. Goodwin, and E. J. Leonard. 1980. A 48-well micro chemotaxis assembly for rapid and accurate measurement of leukocyte migration. J. Immunol Methods 33:(3)239-247; Yang, D., Q. Chen, S. Stoll, X. Chen, O. M. Howard, and J. J. Oppenheim. 2000. Differential regulation of responsiveness to fMLP and C5a upon dendritic cell maturation: correlation with receptor expression. J. Immunol. 165:(5)2694-2702). Briefly, different concentrations of 26 ml chemotactic factors or aliquots of sFv fusion protein, serially diluted in chemotaxis medium (RPMI 1640, 1% BSA, 25 mM HEPES), were placed in the lower compartment of the chamber (Neuro Probe, Cabin John, Mass.), and 50 μl of dendritic cells (10⁶ cells/ml) were added to wells of the upper compartment. The lower and upper compartments were separated by a 5-μm polycarbonate filter (Osmonics, Livermore, Calif.). After incubation at 37° C. in humidified air with 5% CO₂ for 1.5 h, the filters were removed, scraped, and stained. Dendritic cells migrating across the filter were counted with the use of a Bioquant semiautomatic counting system. The results are presented as chemotactic index (C. I.) defined as the fold increase in the number of migrating cells in the presence of test factors over the spontaneous cell migration (in the absence of test factors). The results are expressed as the mean±SE of triplicate samples. MIP-3a and MIP-30 were purchased from PeproTech (Rocky Hill, N.J.).

Chemokine Receptor Binding Assay.

Binding assays were performed by using a single concentration of radio-labeled MIP-1β or SDF-1a (human [¹²⁵-I]-[Leu³, Gly⁴⁷]-MIP-1β and human [¹²⁵I]-SDF-1α,2200 Ci/mmol, NEN Life Science Products Inc., Boston, Mass.) in the presence of increasing concentrations of unlabeled ligands (MIP-1β and SDF-1α obtained from PeproTech, Rocky Hill, N.J.). Human HEK293 cells transfected with CCR5 at 1×10⁶/sample were suspended in 200 μl binding medium composed of RPMI1640, 1 mg/ml BSA, 25 mM HEPES, and 0.05% sodium azide, and incubated in duplicates at room temperature for 40 min. After incubation, the cells were pelleted through a 10% sucrose/PBS cushion and the radioactivity associated with cell pellets was determined in a γ-counter (Clinigamma-Pharmacia, Gaithersburg, Md.). The binding data were then analyzed with a Macintosh computer program LIGAND (P. Munson, Division of Computer Research and Technology, NIH, Bethesda, Md.). The degree of competition for binding by unlabeled chemokines was calculated as follows: % competition for binding=1−(cpm obtained in the presence of unlabeled ligand/cpm obtained in the absence of unlabeled ligand)×100%.

HIV-1 env Antibody and CTL Assays.

Five BALB/c female mice per group were gene-gun immunized with DNA plasmids four times using gene-gun. Two weeks after the last immunization, HIV-189.6 env specific CTL was assessed in spleens and Peyer's patches as described elsewhere (Belyakov, I. M., M. A. Derby, J. D. Ahlers, B. L. Kelsall, P. Earl, B. Moss, W. Strober, and L. A. Berzofslcy. 1998. Mucosal immunization with HIV-1 peptide vaccine induces mucosal and systemic cytotoxic T lymphocytes and protective immunity in mice against intrarectal recombinant HIV-vaccinia challenge. Proc. Natl. Acad. Sci. U.S.A 95:(4)1709-1714). Briefly, immune cells from spleen or Peyer's patch were cultured at 5×10⁶ per/milliliter in 24-well culture plates in complete T cell medium (CTM): RPMI 1640 containing 10% fetal bovine serum, 2 mM L-glutamine, penicillin (100 U/ml), streptomycin (100 mg/ml), and 5×10⁻⁵ M 2-mercaptoethanol. Three days later 10% concanavalin A supernatant was added as a source of IL-2 (T-STIM, Collaborative Biomedical Products, Bedford, Mass.). Spleen or Peyer's patch cells were stimulated in vitro with P18-89.6A9 peptide (IGPGRAFYA; SEQ ID NO:39) (Belyakov, I. M., L. S. Wyatt, J. D. Ahlers, P. Earl, C. D. Pendleton, B. L. Kelsall, W. Strober, B. Moss, and J. A. Berzofsky. 1998. Induction of a mucosal cytotoxic T-lymphocyte response by intrarectal immunization with a replication-deficient recombinant vaccinia virus expressing human immunodeficiency virus 89.6 envelope protein. J. Virol. 72:(10)8264-8272) for a 7-day culture periods before assay. Cytolytic activity of CIL lines was measured by a 4-hour assay with ⁵¹Cr-labeled P815 cell targets. For testing the peptide specificity of CTL, ⁵¹Cr-labeled P815 targets were pulsed for 2 hours with peptide at the beginning of the assay or left unpulsed as controls. The percent specific ⁵¹Cr release was calculated as 100× (experimental release-spontaneous release)/(maximum release−spontaneous release). Maximum release was determined from supernatants of cells that were lysed by addition of 5% Triton-X 100. Spontaneous release was determined from target cells incubated without added effector cells (Belyakov, I. M., M. A. Derby, J. D. Ahlers, B. L. Kelsall, P. Earl, B. Moss, W. Strober, and J. A. Berzofsky. 1998. Mucosal immunization with HIV-1 peptide vaccine induces mucosal and systemic cytotoxic T lymphocytes and protective immunity in mice against intrarectal recombinant HIV-vaccinia challenge. Proc. Natl. Acad Sci. U.S.A 95:(4)1709-1714).

Serum anti-env antibodies assessed by ELISA on 5 μg/ml gp120 protein from isolate 89.6 produced in vaccinia virus coated 96-well plate. The bound antibodies were detected by goat anti-mouse Ig-HRP mAb (Caltag) and developed with ABTS peroxidase substrate (KPL, Gaithersburg, Md.).

Tumor Cell Lines and Mice.

The carcinogen-induced, C3H 38C-13 B cell lymphoma (Bergmanm Y. and J. Haimovich. 1977. Characterization of a carcinogen-induced murine B lymphocyte cell line of C3H/eb origin. J. Immunol. 7:413-417) was obtained from R. Levy (Stanford, Calif.). The 38C-13 tumor secretes and expresses IgM (k) on the cell surface. Inoculation of as few as 10² 38C-13 tumor cells i.p. into normal syngeneic mice results in progressive tumor growth and death of the host with a median survival time of only two weeks. Mice surviving past 60 days from tumor challenge are long-term survivors. The BALM A20 lymphoma (Kim, K. J., L. C. Kanellopoulos, R. M. Merwin, D. H. Sachs, and R. Asofsky. 1979. Establishment and characterization of BALB/c lymphoma lines with B cell properties. J. Immunol. 122:(2)549-554) was obtained from the American Type Culture Collection (Rockville, Md.) and expresses IgGk. 38C-13 and A20 cells from a common frozen stock were passaged in vitro 3 days before use in RPMI 1640 supplemented with 100 U/ml of penicillin and streptomycin, 2×10⁻⁵ M 2-mercaptoethanol, and heat inactivated 10% fetal bovine serum (Gibco BRL, Gaithersburg, Md.).

In Vivo Immunizations and Tumor Protection Experiment.

Animal care was provided in accordance with the procedures outlined in a Guide for the Care and Use of Laboratory Animals (NIH Publication No. 86-23, 1985). Six- to nine-week old female C3H/HeNCrlBR or BALB/c mice (Charles River Laboratories, Frederick, Md.) were used. Syngeneic C3H/HeN or BalbC mice (10 per group) were immunized with Hellos Gene Gun System (Bio-Rad, Hercules, Calif.) with plasmid DNA three times every two weeks . The abdominal area of mice was shaved, and 1μ gold particles (Bio-Rad, Hercules, Calif.) carrying 1-3 μg DNA were injected at 400 psi. Two weeks after the last immunization, mice were challenged i.p. with 2000 38C-13 lymphoma cells from a single preparation of tumor and followed for survival. Differences in survival between groups were determined by non-parametric logrank test (BMDP statistical software, Los Angeles). P-values refer to comparison with group immunized with DNA expressing the same chemokine or defensin fused with an irrelevant sFv, or sFv fused with mutant chemokine, unless specified.

Therapy of Established Tumor with DNA Vaccine.

Six- to nine-week old female BALB/c mice (ten per group) were challenged with 2.5×10³ syngeneic A20 tumor cells. At day 1, 4, 8 and 18 these mice were gene-gun immunized with DNA plasmid (containing about 1-2 μg DNA per immunization) and mice followed for tumor progression.

Results

Property of Constructs: Murine β-Defensins and Viral Chemokines Retain their Functional Integrity when Produced as Fusion Proteins with sFv.

First, a variety of chemokine and β-defensin fusion proteins with sFv, a lymphoma Ig-derived non-immunogenic Fv, were cloned and purified (Table 1). The functional integrity of these proteins were tested by the ability to induce chemotaxis of murine APC and THP-1 cells. As expected, chemokine fusion proteins induced dose-dependent chemotaxis. THP-1 cells were chemo-attracted to vMIP1, human MCP-3, and SDF-10 fusion proteins, but not to the fusion with antagonist chemokine vMIP2, vMIP2sFv38. Control mutant fusion proteins generated for the each chemokine by replacing the first Cys residue by Ser or by truncation of the amino-termini, as expected, did not induce chemotaxis of THP-1 cells or murine DC. Furthermore, vMIP2 fusion proteins were tested for their ability to bind to their respective receptor (−s). vMIP2sFv38 could displace labeled MIP1β and SDF1α, in a dose dependent manner from CCR5 and CXCR4 transfected cell lines, respectively. In contrast, no displacement was detected by vMIP2MsFv38 fusion protein, which contained a replacement Cys/Ser mutation in vMIP2 or by control sFv protein alone.

Since human β-defensin 2 was reported to act via CCR6, murine β-defensin fusion proteins were assayed for their ability to induce chemotaxis of different subsets of murine cells. β-defensin fusion proteins induced chemotaxis of murine bone marrow derived iDC in a dose dependent manner with peak activity at 10 ng/ml and 100 ng/ml for Def2βsFv38 and Def3βsFv38, respectively. The immature phenotype of these DC (see Methods) was also supported by their ability to migrate to human MIP3α, a chemo-attractant specific for CCR6⁺ immature DC (Dieu, M. C., B. Vanbervliet, A. Vicari, J. M. Bridon, E. Oldham, S. Ait-Yahia, F. Briere, A. Ziotnik, S. Lebecque, and C. Caux. 1998. Selective recruitment of immature and mature dendritic cells by distinct chemokines expressed in different anatomic sites. J. Exp. Med 188:(2)373-386; Yang,

TABLE 1 Ligand-Antigen fusion constructs DNA vaccine Ligand: Defensin or name chemokine Antigen Protein Name Description Antigen alone psFv38 none sFv38 sFv38 Single chain antibody fragment from 38C-13 lymphoma psFv20 none sFv20 sFv20 Single chain antibody fragment from A20 lymphoma pgp120 none gp120 gp120 gp120 antigen (HIV-1, isolate 89.6) Defensin fusions: pmDF2βsFv38 murine β-defensin 2 sFv38 mDF2βsFv38 Murine β-defensin 2 fusion with sFv38 pmDF2βgp120 murine β-defensin 2 gp120 mDF2βgp120 Murine β-defensin 2 fusion with gp120 (HIV-1, 89.6) pmDF3βsFv38 murine β-defensin 3 sFv38 mDF3βsFv38 Murine β-defensin 3 fusion with sFv38 pproDF2βsFv38 murine pro-β-defensin 2 sFv38 mproDF2βsFv38 Murine pro-β-defensin 2 fusion with sFv38 Viral chemokine Fusions: pvMIP2sFv38 viral MIP2 sFv38 vMIP2sFv38 Viral MIP2 fusion with sFv38 pvMIP1sFv38 viral MIP1 sFv38 vMIP1sFv38 Viral MIP1 fusion with sFv38 pMC148sFv38 MC148 sFv38 MC148sFv38 Viral MC148 fusion with sFv38 Pro-inflammatory Chemokine fusions: phMCP3sFv38 Human MCP-3 sFv38 hMCP3sFv38 Human MCP-3 fusion with sFv38 phMCP3sFv20 Human MCP-3 sFv20 hMCP3sFv20 Human MCP-3 fusion with sFv20 phMCP3gp120 Human MCP-3 gp120 hMCP3gp120 Human MCP-3 fusion with gp120 (HIV-1, isolate 89.6) phMDCsFv38 Human MDC sFv38 hMDCsFv38 Human MDC fusion with sFv38 phMDCsFv20 Human MDC sFv20 hMDCsFv20 Human MDC fusion with sFv20 phMDCgp120 Human MDC gp120 hMDCgp120 Human MDC fusion with gp120 (HIV-1, isolate 89.6) phSDF1βsFv38 Human SDF-1β sFv38 hSDF1βsFv38 Human SDF1-β fusion with sFv38 Mutant chemokine fusions: pvMIP2MsFv38 Mutant vMIP2 sFv38 vMIP2MsFv38 Mutant vMIP2 fusion with sFv38 pvMIP1MsFv38 Mutant vMIP1 sFv38 vMIP1MsFv38 Mutant vMIP1 fusion with sFv38 phMCP3MsFv38 Mutant hMCP-3 sFv38 hMCP3MsFv38 Mutant human MCP-3 fusion with sFv38 phMDCMsFv38 Mutant hMDC sFv38 hMDCMsFv38 Mutant human MDC fusion with sFv38 Control fusions: pmDF3βMuc1 β-defensin 3 Muc-1 mDF3βMuc1 Murine β-defensin 3 fusion with 80 aa hMuc-1 peptide phMCP3-EGFP Human MCP-3 EGFP hMCP3-EGFP Human MCP-3 fusion with EGFP protein phMDC-EGFP Human MDC EGFP hMDC-EGFP Huma MDC fusion with EGFP protein Protein vaccine: Ig38-KLH None Ig38 Ig38-KLH 38C-13 lymphoma derived IgM protein cross-linked with KLH Ig20-KLH none Ig20 Ig20-KLH A20 lymphoma derived IgG2a protein cross-linked with KLH

D., O. M. Howard, Q. Chen, and J. J. Oppenheim. 1999. Cutting edge: immature dendritic cells generated from monocytes in the presence of TGF-beta 1 express functional C—C chemokine receptor 6. J. Immunol 163:(4)1737-1741), and their inability to react to human MIP3β (Sallusto, F., B. Palermo, D. Lenig, M. Miettinen, S. Matikainen, I. Julkunen, R. Forster, R. Burgstahler, M. Lipp, and A. Lanzavecchia. 1999. Distinct patterns and kinetics of chemokine production regulate dendritic cell function. Eur. J. Immunol 29:(5)1617-1625), a chemo-attractant specific for CCR7⁺ mature DC. None of the defensin fusion proteins stimulated chemotaxis of mature DC, which migrated to MIP3β. Control fusion protein proDef2βsFv38 did not induce chemotaxis of any DC. Therefore, murine β-defensin 2 and 3 fusion proteins can specifically target immature DC. Furthermore, sFv fusion with β-defensin and xenogeneic human or viral chemokines does not disrupt their functional chemokine properties.

Murine β-Defensin, Xenogeneic Proinflammatory and Viral Chemokine Fusion Constructs Render Non-Immunogenic Tumor Antigen Immunogenic.

Next, these fusion proteins were used to induce specific immunity against non-immunogenic sFv38 when administered as a DNA vaccine in mice. Ten mice per group were immunized by gene-gun with plasmids encoding fusion proteins with mature β-W defensins, pDef2βsFv38 and pDef3βsFv38, respectively, or with human or viral chemokines, pSDF1βsFv38, pMDCsFv38, pvMIP1sFv38 or pvMIP2sFv38. Control mice were immunized with DNA constructs encoding sFv fused with inactive pro-Defensin (pproDef2βsFv38), or mutated chemokines (phMCP3MsFv38, pMDCMsFv38, pMIP1MsFv38 and pvMIP2MsFv38). Mice immunized with plasmids encoding sFv fusion proteins with both murine β-defensins, murine MCP-3, human MDC or viral chemokines induced significant idiotype-specific antibodies which were comparable to the levels induced by vaccination with tumor-derived intact Ig protein conjugated to KLH. In contrast, control mice immunized with an inactive pro-β-defensin (pproDef2βsFv38) or mutant chemokine sFv fusion constructs (hpMCP3MsFv38, pMDCMsFv38 and pvMIP2MsFv38), or sFv38 alone did not produce any anti-Id antibody responses. Moreover, a mixture of separate plasmids encoding β-defensin 3 (pmDF3βMuc1T) and sFv antigen (sFv38) failed to elicit a specific humoral response, demonstrating a requirement for sFv to be physically linked to β-defensin or chemokine moiety. Therefore, non-immunogenic sFv was rendered immunogenic by fusion with mature murine β-defensins, syngeneic murine, xenogeneic human or viral chemokines. These results also suggest that it was not sufficient to simply attract APC to the site of production of sFv, but that direct APC targeting with self-antigen fused to β-defensin or chemokine was required. Thus, induction of anti-Id antibodies by sFv fusion proteins appeared to involve receptor-mediated binding and delivery of antigen to APC. Vaccination elicited anti-Id antibodies of various isotypes, suggesting activation of different effector cells by different pro-inflammatory moieties. All carriers induced specific IgG1 antibodies. However, MDC containing vaccines also elicited high titers of IgG2b and IgG3, while fusion constructs with β-defensin-3 and vMIP2 elicited high titers of IgG2b but little IgG3, and little IgG2b or IgG3, respectively.

Two weeks after the last of three serial immunizations, mice were challenged with a 20-fold lethal dose of syngeneic tumor. No survival was observed in control groups immunized with PBS or plasmids encoding sFv38 fused with inactive pro-β-defensin-2 (pproDef2βsFv38), MDC alone (pMDC-EGFP), or with mutant constructs pMDCMsFv38, pvMIP2MsFv38, pvMIPIMsFv38. Moreover, no protection was observed in mice immunized with DNA encoding a mixture of unlinked functionally active β-defensin or chemokine with sFv. In contrast, significant protective immunity was elicited in mice immunized with pDef2βsFv38 and pDef3βsFv38 (logrank P<0.001 as compared with pproDef2(3sFv38 and pMIP2MsFv38, respectively). Similarly, pMDCsFv38, pvMIP2sFv38 and pvMIP1sFv38 immunized mice demonstrated statistically significantly prolonged survival (logrank P<0.001 as compared with pMDC-EGFP and mutant pvMIP2MsFv38 and pvMIP1MsFv38, respectively). Therefore, β-defensins and xenogeneic human and viral chemokines can render a non-immunogenic self-rumor antigen (sFv) immunogenic and elicit specific antitumor immunity. These data also suggest that chemokine receptor engagement with chemokine- or defensin-sFv fusion is useful for the induction of immunity.

Requirement for Secretion but not for Chemotaxis for Induction of Immune Responses.

Additional constructs were used for testing in vivo. Mice were immunized with MCP-3 fusion constructs with or without a secretory leader sequence (pMCP3sFv38 and pMCP3sFv38-w/o-SL, respectively). High levels of Id-specific antibodies were detected in mice immunized with pMCP3sFv38, containing an intact secretory leader; however, no antibodies were elicited in mice immunized with pMCP3sFv38-w/o-SL. Furthermore, tumor protection was elicited only in those mice immunized with pMCP3sFv38, but not with pMCP3sFv38-w/o-SL (logrank P<0.001). In addition, no protection was detected in mice immunized with DNA expressing a secretable but mutated MCP-3 fusion protein, which could not bind the respective receptor (pMCP3MsFv38). These data are consistent with immunity being induced by APC which took up (via chemokine receptor) a functionally active chemokine fusion protein which was secreted from bystander cells, rather than by APC directly being transduced by gene gun immunization.

It was determined whether activation of receptor-mediated chemotaxis was required for eliciting immune responses, or whether receptor binding alone was sufficient. Immune responses of a selective pair of agonist (vMIP1) (Endres, M. J., C. G. Garlisi, H. Xiao, L. Shan, and J. A. Hedrick. 1999. The Kaposi's sarcoma-related herpesvirus (KSHV)-encoded chemokine vMIP-1 is a specific agonist for the CC chemokine receptor (CCR)8. J. Exp. Med. 189:(12)1993-1998) and antagonist (MC148) (Luttichau, H. R., J. Stine, T. P. Boesen, A. H. Johnsen, D. Chantry, J. Gerstoft, and T. W. Schwartz. 2000. A highly selective CC chemokine receptor (CCR)8 antagonist encoded by the poxvirus molluscum contagiosum. J. Exp. Med. 191:(1)171-180) chemokines, which bind to CCR8, were compared to immune responses in mice immunized with plasmids encoding pvMIP1 and MC148 fusion proteins, respectively (pMIP1sFv38 and pMC148sFv38): Mice immunized with either of these chemokine fusion constructs produced comparable levels of specific antibodies. Moreover, significant tumor protection was detected in both groups of mice challenged with a high dose of 38C-13 cells (logrank P<0.001 for pMC148sFv38 and P<0.01 for pvMIPIsFv38, respectively, compared with control pvMIP1MsFv38). These data suggest that chemokine receptor binding alone, in the absence of subsequent signaling for chemotaxis, is sufficient to induce immunity.

Discussion

This example demonstrates that use of proinflammatory factors of innate and adaptive immunity such as β-defensins 2 and 3 and viral chemokines (Luster, A. D. 1998. Chemokines—chemotactic cytokines that mediate inflammation. N. Engl. J. Med. 338:(7)436-445) can help to elicit strong immune responses both against a model non-immunogenic tumor antigen, lymphoma idiotype (Stevenson, F. K., D. Zhu, C. A. King, L. J. Ashworth, S. Kumar, and R. E. Hawkins. 1995. Idiotypic DNA vaccines against B-cell lymphoma. Immunol. Rev. 145:211-228), and viral antigen, HIV gp120. The appeal of this approach was based not only on the ability of these mediators of innate and adaptive immunity to target surface receptors on APC, particularly on iDC (Yang, D., O. Chertov, S. N. Bykovskaia, Q. Chen, M. J. Buffo, J. Shogan, M. Anderson, J. M., Schroder, I. M. Wang, O. M. Howard, and J. J. Oppenheim. 1999. Beta-defensins: linking innate and adaptive immunity through dendritic and T cell CCR6. Science 286:(5439)525-528), presumably resulting in increased uptake of antigen, but possibly also to induce of expression of co-stimulatory molecules and, in turn, production of other pro-inflammatory cytokines and factors. This example demonstrates that both murine β-defensin 2 and 3 efficiently induced chemotaxis of immature, but not mature, murine bone marrow derived DC, suggesting that a β-defensin specific receptor(s) is expressed on immature DC.

Example 4

As an example of how the vaccine of this invention can be administered to a patient to treat cancer or to treat or prevent HIV infection (with the additional administration of adjuvants, such as immunostimulatory cytokines, if desired), the following is a complete protocol for a clinical trial describing the administration of Id-KLH and GM-CSF to patients to treat follicular lymphoma. The same study design can be employed for the administration of the viral chemokine-tumor antigen fusion polypeptide or the viral chemokine-viral antigen fusion polypeptide of the present invention or nucleic acids encoding the fusion polypeptides of this invention, with appropriate modifications, as would be apparent to one of skill in the art. In particular, studies to test the efficacy of HIV vaccines are well known in the art and the clinical protocol described herein can be readily modified by one of skill in the art as appropriate to test the efficacy of the HIV fusion polypeptide or HIV fusion polypeptide-encoding nucleic acid of this invention according to well known protocols for testing HIV vaccines (126,127).

Background and Rationale

Immunoglobulin (Ig) molecules are composed of heavy and light chains, which possess highly specific variable regions at their amino termini. The variable regions of heavy and light chains combine to form the unique antigen recognition site of the Ig protein. These variable regions contain determinants that can themselves be recognized as antigens, or idiotopes. B-cell malignancies are composed of clonal proliferations of cells synthesizing a single antibody molecule with unique variable regions in the heavy and light chains. B-cell lymphomas are neoplasms of mature resting and reactive lymphocytes which generally express synthesized Ig at the cell surface. The idiotypic determinants of the surface Ig of a B-cell lymphoma can thus serve as a tumor-specific marker for the malignant clone.

Studies in experimental animals, as well as in man, have demonstrated the utility of the Ig idiotype as a tumor-specific antigen for the study of the biology of B-cell lymphoma in vitro and as a target for passive immunotherapy in vivo (1, 2, 3). Furthermore, active immunization against idiotypic determinants on malignant B cells has been demonstrated to produce resistance to tumor growth in a number of syngeneic experimental tumor models, as well as specific anti-tumor therapy against established tumors (4-13). These results, taken together, provided the rationale for testing autologous tumor-derived idiotypic surface Ig (Id) as a therapeutic “vaccine” against human B-cell lymphoma. Furthermore, preclinical studies in subhuman primates demonstrated that optimal immunization with human lymphoma-derived Id required conjugation of the protein to an immunogenic protein carrier (keyhole limpet hemocyanin; KLH) and emulsification in an adjuvant (14).

Guided by these observations, nine patients with B-cell lymphoma were immunized with autologous Id protein (15). These patients received no anti-tumor therapy during the time of the study. They were either in complete remission or in a state of minimal residual disease following conventional chemotherapy. In addition, three patients with rapidly progressive recurrent lymphoma were enrolled in a separate safety study; all three required reinstitution of chemotherapy shortly after enrollment, did not complete the immunization series, and were not studied further. They received intramuscular injections of 0.5 mg of Id conjugated to KLH at 0, 2, 6, 10 and 14 weeks, followed by two booster injections at 24 and 28 weeks. Patients in the first trial (five patients) received Id-KLH alone for the first three immunizations, then Id-KLH emulsified in a Pluronic polymer-based adjuvant vehicle formulation for all subsequent immunizations. Because no idiotype-specific immune responses were observed prior to the addition of the adjuvant to the program in this first group of patients, patients in the second trial (four patients) received the entire series of immunizations with this adjuvant. All patients were analyzed for idiotype-specific antibody production and peripheral blood mononuclear cell (PBMC) proliferative responses in vitro immediately before each immunization and at one to two month intervals following the last immunization. The KLH carrier provided a convenient internal control for immunocompetence of the patients and all patients demonstrated both humoral and PBMC proliferative responses to the KLH protein, with the exception of one patient, who demonstrated only the latter. Seven of the nine patients demonstrated either a humoral (n=2) or a cell-mediated (n=4) anti-idiotypic immunological response, or both (n=1).

Anti-idiotypic antibody responses were detected by analysis of pro- and hyper-immune sera in either direct, or competition, ELISA. The immunization with autologous Id protein induced significant titers of anti-idiotypic antibody that either directly bound or inhibited the binding of a murine anti-idiotype monoclonal antibody (anti Id mAb) to Id on the plate. The specificity of the humoral response for the Ig idiotype was demonstrated by the lack of significant binding of hyperimmune serum to a panel of isotype-matched human Igs of unrelated idiotype, or by the lack of significant inhibition of a panel of heterologous Id-anti-Id systems, respectively. Peak humoral responses were obtained after the fifth immunization and persisted for at least nine months. The anti-idiotypic antibody produced by patient 1 was affinity-purified and shown to contain heterogeneous light chains as well as immunoglobulin G heavy chains. This patient's antibody titer was successfully boosted with a single administration of Id-KLH in adjuvant after a decline of the humoral response after 15 months.

Cellular immune responses were measured by the proliferation of PBMC to KLH and to autologous Id separately at concentrations ranging from 1-100 μg per milliliter of soluble protein in five day in vitro cultures. None of the pre-immune PBMC demonstrated any preexisting proliferation to autologous Id above that to culture medium alone. Hyperimmune PBMC from all patients demonstrated strong proliferative responses to the KLH carrier. Of primary interest, significant hyperimmune proliferative responses to Id were detected in five patients. Although their responses were of lower magnitude than parallel responses to KLH, patients 3, 4, 6, 8 and 9 were classified as responders on the basis of reproducible increases in counts-per minute (cpm) ³H-thymidine incorporation in wells containing Id, compared with medium alone, that were sustained over multiple time points. Patients demonstrating occasional increases in cpm in wells containing Id compared with medium alone were classified as non-responders (patients 1 and 5).

Flow cytometry analysis of cultures demonstrating proliferation to Id revealed a predominance of cells staining positively for CD4 (>95%), suggesting the phenotype of the responding cell subpopulation. These cultures could be successfully expanded for approximately four weeks by stimulation alternatively with interleukin-2 (IL-2) and Id-pulsed autologous irradiated PBMC as antigen-presenting cells. Specificity of the responses for Ig idiotype was confirmed by the lack of significant proliferation to an isotype-matched human Ig of unrelated idiotype compared with medium alone. Such idiotype-specific PBMC proliferative responses were observed only after the addition of the adjuvant to the program and also persisted for at least 9-14 months.

The ability of the idiotype-specific humoral response to bind autologous tumor cells was also tested. This was shown by the inhibition of binding of a labeled murine anti-idiotype mAb to tumor cells from a pre-treatment lymph-node specimen from patient 8 by hyperimmune, but not by pre-immune, serum from this patient. In addition, affinity purified anti-idiotypic antibodies from the hyperimmune sera of the two other patients who demonstrated idiotype specific humoral responses were demonstrated by flow cytometry to bind autologous tumor.

All patients were also closely monitored for disease activity with physical examinations and routine laboratory and radiographic studies. Of the two patients with measurable tumor at the initiation of Id immunization, one (patient 1) experienced complete regression of a single 2.5 cm left submandibular lymph node, and the other (patient 4) experienced complete regression of a 4.5 cm cutaneous lymphomatous mass on the right arm. This clinical response in patient 4 correlated with an Id-specific, PBMC proliferative response in vivo. Correlating with the duration of their immunological responses, the clinical responses in both patients have continued at 24 and 10 months, respectively, after completion of the immunization series. Moreover, with a median follow up time of 10 months, the only case of tumor recurrence among those patients who were in remission and completed the immunization series occurred in patient 5, who was one of the two patients who failed to demonstrate an idiotype-specific immunological response.

Toxicity was minimal in all twelve patients. All patients experienced transient local reactions characterized by mild erythema, induration, and discomfort, without skin breakdown, at the injection sites. Splitting the components of the vaccine (Id-KLH and adjuvant) in one patient who had experienced a moderate local reaction and in another patient who had experienced a moderate systemic reaction, characterized by fever, rigors and diffuse arthralgias, established the adjuvant as the component associated with these reactions. Both of these moderate reactions resolved completely after 24-48 hours. The only laboratory abnormality associated with Id immunization was a mild elevation (less than twice the normal value) of serum creatine phosphokinase 24 hours after immunization in an occasional case.

These results demonstrate that patients with B-cell lymphoma can be induced to make sustained idiotype-specific immune responses by active immunization with purified autologous tumor-derived surface Ig. They show that autologous Id, made immunogenic by conjugation to KLH, can serve as an immunogen (antigen) to elicit host immunological responses. The induction of low levels of idiotype-specific immunity was demonstrated in the setting of minimal tumor burden following conventional chemotherapy. These results, taken together with the induction of relatively stronger immune responses to the KLH carrier, and exogenous antigen, suggest that chemotherapy-induced immunosuppression is not an obstacle to active immunotherapy administered adjunctively to cytoreductive drug therapy in this manner.

This initial study also established the requirement for an immunological adjuvant, as no Id-specific responses were observed prior to the addition of an adjuvant to the program. The objective of further clinical trials using tumor derived Id as a therapeutic vaccine is to further optimize the immunogenicity of this vaccine. To this end, this study will focus on the use of novel immunological adjuvants which are 1) more potent and 2) more effective in the induction of cell-mediated immune responses, compared with the pluronic polymer-based adjuvant used in the study.

The 38C13 B cell tumor is used as a model system to screen promising immunological adjuvants. A number of these have included cytokines and among these, GM-CSF has emerged as a promising adjuvant for idiotypic Ig antigen. In these experiments (10 mice per group), syngeneic mice were immunized with 50 μg Id-KLH derived from the tumor, either alone or in combination with GM-CSF mixed together with the antigen and administered subcutaneously. Three additional daily doses of GM-CSF were administered s.c. as close to the original site of immunization as possible. Mice immunized with an irrelevant Id-KLH (4C5 IgM) served as negative controls for the vaccine. Two weeks after this single immunization, all mice were challenged with a single preparation of 38C13 tumor cells (5×10³ cells i.p.) and followed for survival. The results demonstrated that the augmented survival benefit afforded by immunization with relevant Id-KLH alone can be significantly enhanced by the addition of GM-CSF at either the 100 or 10,000 unit dose. The loss of this protective effect at a higher dose of GM-CSF of 50,000 units was also observed. These data suggest that GM-CSF may have a potent adjuvant effect in vivo for Id-KLH antigen, especially at relatively low doses.

The follicular lymphomas are follicular small cleaved cell (FSC) and follicular mixed lymphoma (FM). Stage I and II patients comprise only 10% to 15% of all cases of follicular lymphomas and are best managed with radiation therapy. Eight-five percent of patients with follicular lymphomas present with stage 111 or IV disease. The optimal management of these patients remains controversial and has generally followed two divergent approaches (16, 17). One is an aggressive approach, which has included radiation therapy, combination chemotherapy, or combined modality therapy and the other is a conservative approach that involves no initial treatment followed by a single-agent chemotherapy or involved-field radiotherapy when required (18; 19). Most forms of systemic therapy have the capacity to produce high complete response rates. However, they have failed to produce long-term disease-free survival or to prolong overall survival; thus, it has become clear that the vast majority of patients with this disease will relapse and die of their lymphoma, despite its usually indolent course.

The NCI study (MB-110, BRMP 8903) begun in 1978, is a prospective randomized study comparing these two distinct approaches to the management of stage III or IV indolent histology lymphoma. Most patients were randomized between no initial therapy or aggressive combined modality therapy with ProMACE/MOPP flexitherapy followed by low dose (2400 cGy) total nodal irradiation. Among the 149 patients treated thus far, 125 (84%) were randomized; 62 to watch and wait (W & W) and 63 to aggressive treatment. Among the 62 patients on the watch and wait arm, 29 continue to be observed for periods up to 10+ years. The median time to cross over to aggressive therapy is 23 months.

It is apparent that patients in whom therapy is initiated after the development of symptoms have a significantly lower complete response rate to therapy than patients randomized to receive the same therapy at diagnosis (74% vs 40%, P₂=0.0039). The complete responder (CR) rate of patients randomized to initial aggressive treatment is comparable to those obtained in patients with advanced-stage intermediate grade lymphoma receiving the same treatment. The CR rate in indolent lymphoma does not appear to be significantly higher than what can be achieved with other combination regimens. For patients randomized to watch and wait, median follow-up of CRs is shorter because of the delay in initiating treatment. However, the median duration of remission has not been reached at five years and 57% of patients are projected to be disease-free >8 years and 44% are projected to be in a CR at 12 years. The disease-free survival curves are not significantly different between the two arms. Thus, allowing the patient to reach a greater tumor burden before instituting systemic therapy reduces the likelihood of obtaining a CR, but once achieved, CRs are comparably durable to those obtained from primary aggressive therapy. The lengthening of the remission duration, however, has not resulted in a survival advantage for patients randomized to receive primary aggressive chemotherapy. Furthermore, even though a minority of complete responders have relapsed, the probability of relapse appears to be continuous over time, and the vast majority of patients are expected to eventually succumb to their disease.

Thus, even immediate aggressive therapy has not resulted in improved survival. Therefore, although patients diagnosed with follicular lymphoma enjoy relatively longer survival times compared with patients with solid tumors, follicular lymphoma remains an incurable disease. Novel experimental therapies designed to improve the durability of the remissions already effectively induced by chemotherapy are justified.

Summary of Treatment Plan

The goal is to treat patients with follicular lymphomas to complete remission or maximal response with ProMACE chemotherapy. After the completion of chemotherapy, in an effort to reduce the relapse rate (by eradicating microscopic disease resistant to chemotherapy), patients will receive an autologous Id vaccine administered in combination with GM-CSF.

The goal of this study is to evaluate the ability of the Id vaccine to clear the bone marrow of malignant cells detectable by pathologic (morphologic) examination or molecular examination (polymerase chain reaction, PCR) in patients with PCR amplifiable translocations. All patients have serial bone marrow and peripheral blood samples collected to search for clonal abnormalities by PCR. Patients are followed after vaccine therapy and their remission status correlated with clinical vs. molecular determinations of response. There should be three categories of complete responders: those who had a clinical complete response before the vaccine but had an abnormal clone by PCR that cleared after the vaccine; those with a clinical CR before the vaccine who were also PCR negative before the vaccine; and those who achieved a clinical complete response but had PCR positive marrows before and after the vaccine. It is a goal of this study to assess whether “molecular complete responses” can be achieved using the vaccine in patients following chemotherapy.

Objectives

The objectives of this trial are to:

To induce cellular and humoral immunity against the unique idiotype expressed on the surface of patients' B-cell lymphomas.

To determine the ability of Id immunization to eradicate bcl-2 positive tumor cells from the bone marrow as detected by PCR.

As a secondary objective, to determine the more biologically active of the two GM-CSF doses as an adjuvant, as measured by the endpoints in the above objectives.

To determine the impact of Id immunization on disease free survival of patients achieving a CR with chemotherapy.

Patient Selection Patient Sample

A. Sample size, approximately 42 patients

B. Sex distribution: male and female

C. Age: patients must be ≧18 years old

Eligibility Criteria

-   -   Patient must meet all of the following eligibility criteria:     -   A. Tissue diagnosis of: follicular small cleaved cell, or         follicular mixed lymphoma with surface IgM, IgG or IgA phenotype         with a monoclonal heavy and light chain. Pathology slides must         be submitted to the NIH Pathology Department for review.     -   B. Stage III or IV lymphoma.     -   C. Only previously untreated patients are eligible.     -   D. Previous treatment with radiation alone (less than TBI) is         permissible.     -   E. A single peripheral lymph node of at least 2 cm size         accessible for biopsy/harvest.     -   F. Karnfsky status a ≧70%.     -   G. Life expectancy of >one year.     -   H. Serum creatinine ≦1.5 mg/dl unless felt to be secondary to         lymphoma.     -   I. Bilirubin ≦1.5 mg/dl unless felt to be secondary to lymphoma         or Gilbert's disease. SGOT/SGPT <3.5× upper limit of normal.     -   J. Ability to give informed consent. Ability to return to clinic         for adequate follow-up for the period that the protocol         requires.

Patient Exclusion Criteria

-   -   The presence of any exclusion criteria (listed below) will         prohibit entry into study:     -   A. Prior total body irradiation.     -   B. Presence of antibodies to HIV, hepatitis B surface antigen or         other active infectious process.     -   C. Pregnancy or lactation. Fertile men and women must plan to         use effective contraception. A beta-HCG level will be obtained         in women of childbearing potential.     -   D. Patients with previous or concomitant malignancy, regardless         of site, except curatively treated squamous or basal cell         carcinoma of the skin, or effectively treated carcinoma in situ         of the cervix.     -   E. Patient unwilling to give informed consent.     -   F. Failure to meet any of the eligibility criteria described         above.     -   G. Any medical or psychiatric condition that in the opinion of         the protocol chairman would compromise the patient's ability to         tolerate this treatment.     -   H. Patient with CNS lymphoma (current or previously treated)         will not be eligible.

Clinical Evaluation

Complete history and physical examination.

CBC, diff., platelet count.

Serum chemistry, β₂-microglobulin.

PT/PTT

Quantitative immunoglobulins, serum protein electrophoresis, immunoelectrophoresis.

HIV antibody, HBsAg.

Urinalysis.

Serum β-HCG in women of child-bearing potential.

EKG and MUGA.

5 TT for serum storage.

Leukapheresis to obtain 3×10⁹ lymphocytes. These samples will be used for baseline studies of T-call activation and response to Id.

Tumor Biopsy—prior to therapy, all patients must undergo biopsy/harvest of a clinically involved peripheral lymph node to obtain tissue for morphological classification, immunophenotypic characterization, determination of immunoglobulin gene rearrangements, bcl-2 translocation, cytogenetics, and to provide starting material for an Id vaccine. The sample should be at least 2 cm in size. Only patients with tumors that are surface immunoglobulin positive with a monoclonal heavy and light chain will be accepted as study candidates. Use standard lymphoma vaccine biopsy orders (see protocol below). Leftover tumor biopsy samples may be used for basic studies of lymphoma biology in vitro. Such future studies may be done without re-consenting the subjects only if the studies involve risks already outlined in the original consent form.

CXR-PA and LAT.

CT scan of abdomen and pelvis.

Lymphangiogram, unless contraindicated by massive pedal edema, severe chronic lung disease, ethiodal sensitivity (Note: sensitivity to other iodine compounds, e.g., renograffin, are relative, but not absolute contraindications).

Other tests (CT chest, ultrasound, liver scan, bone scan, upper and lower GI series, IVP, MRI) should be performed as needed to evaluate all disease sites adequately.

Examination of pleural fluid or ascites when present.

Bilateral bone marrow aspirates and biopsies—In addition to the normal aspirate and biopsy, 5 cc of marrow will be aspirated from each side into 0.5 ml of PFH for PCR analysis. The procedure should be performed in the usual manner with a biopsy performed first. Then a small volume (0.5-1 cc) can be aspirated for the smear and clot tube. A separate Rosenthal needle with bevel should be used for the aspirate. The 5 cc sample for PCR can be obtained from the same site as the initial aspirate.

CT scan of the head and lumbar puncture with CSF analysis if clinically indicated.

Patient Registration

Patients will be registered prior to the initiation of therapy at which time eligibility criteria will be reviewed. Stratification and randomization are described in detail below (see Statistical considerations).

STUDY DESIGN ProMACE Day 0 Day 7 Day 28 Cyclophosphamide Cyclophosphamide Next cycle begins 650 mg/m² IV 650 mg/m² IV Doxorubicin Doxorubicin  25 mg/m² IV  25 mg/m² IV Etoposide VP-1 6 Etoposide BP-1 6 120 mg/m² IV 120 mg/m² IV Prednisone 60 mg/m² po qd × 14 (days 0 to 13) Bactrim one double strength tablet po BID throughout therapy

All patients will be treated until a complete remission is obtained and two additional cycles of chemotherapy have been given, or until disease has been stable for two cycles of chemotherapy, or progressive disease develops. A minimum of six cycles will be given to each complete responder before therapy is discontinued. Patients with more than 90% PR or a full CR will be continued on the vaccination part of the protocol. Patients with less than 90% PR or progressive disease will be taken off of the study.

Postinduction Therapy—Three to six months (or whenever a customized GMP vaccine is available, up to a maximum period of 12 months) after the completion of chemotherapy, all patients in whom either a complete clinical remission or minimal disease status 90% partial response) has been achieved will receive a series of five injections of a vaccine consisting of 0.5 mg autologous tumor derived immunoglobulin (Id) conjugated to KLH. The vaccine will be administered together with GM-CSF as an immunological adjuvant. Both the vaccine and GM-CSF will be administered subcutaneously according to the following schedule:

Schedule: At 0, 1, 2, 3 and 5 months

-   -   Id-KLH (0.5 mg s.c.) day 0     -   adjuvant (s.c.) days 0-3     -   Cohort 1: GM-CSF 500 mcg/m²/d s.c. for 4 days     -   Cohort 2: GM-CSF 100 mcg/m²/d s.c. for 4 days

The sites of injection will be rotated between the upper and lower extremities. Each dose of vaccine or GM-CSF will be split equally between the two upper or lower extremities. All GM-CSP injections will be given in close proximity to the vaccination site, as close to the exact site of injection as possible. If local reactions to GM-CSF are severe, GM-CSF injections may be given elsewhere. Patients will be observed in the clinic for two hours following Id-KLH and/or GM-CSF administration. During the observation period, vital signs will be taken every 15 minutes during the first hour and every 30 minutes during the second hour.

Supportive Care

G-CSF 5 mcg/kg/d SC may be used in all patients who are hospitalized for the treatment of febrile neutropenia, regardless of how long the neutropenia persists.

Grading and Management of Toxicity

Chemotherapy: Dose modification of chemotherapy will be based on the granulocyte count done at the time of drug administration (day 0 or 7 of each cycle). The percentage of drugs administered may be further modified based on toxicity in prior cycles (see below). If the granulocyte count is <1200, and the patient is due for day 0 drugs, delay day 0 for one week until appropriate parameters are met. In general, delays of up to one week are preferable to starting G-CSF. If after a one week delay, appropriate parameters are still not met, then G-CSF may be started as above. Also, in general, delays of up to one week are preferable to dose reductions. Full doses of all drugs should be given on time if blood count suppression is due to bone marrow involvement with disease.

Dose Modification for Hematologic Toxicity

IF GRANULOCYTE COUNT IS: On Day 0 THEN DOSE AS FOLLOWS: ≧1200 100% all drugs ≦1200 Day 0 Delay

For neutrophil nadir <500 or platelet count <25,000 on previous cycle, 75% of cyclophosphamide, doxorubicin, and etoposide should be considered. For neutrophil nadir (day 21 counts)>750 on a previous cycle, dose escalation of cyclophosphamide, doxorubicin, and etoposide by 10-20% should be prescribed.

IF PLATELET COUNT IS: THEN DOSE AS FOLLOWS: >100,000 100% of all drugs 50-99,999 100% Prednisone 75% Etoposide 50% Cyclophosphamide, Doxorubicin  <50,000 Delay

Dose Modification for Non-Hematologic Toxicity

Assessment of non-hematologic toxicity will be graded according to the CRB/DCS/NCI Common Toxicity Criteria. Chemotherapy will be withheld in patients experiencing grade 2 or greater non-hematologic toxicity until the patient has completely recovered from the toxicity. For nausea/vomiting 2: grade 2, drug therapy should be continued with non-steroid antiemetics.

Doxorubicin dosage should be adjusted as follows in the presence of the following LFT abnormalities:

% Dose Bilirubin SGOT 100 <1.5 mg/dl <75 U 50 1.5-2.9 mg/dl 75-150 U 25 3.0-5.9 mg/dl 151-300 U 0 ≧6.0 mg/dl >300 U

Immunotherapy

-   -   Id-KLH Vaccine

Based on previous experience with autologous vaccines, little or no toxicity is expected from the Id-KLH component of the vaccine (15). Nevertheless, any local skin reactions will be carefully noted and scored for erythema, induration, pain and disruption of the barrier surface. If any patient has a reaction suggestive of sensitization, the vaccine may be split into its component parts; specifically, the patient will be tested with Id-KLH alone and then GM-CSF alone. Toxicities will be graded according to the CRBINCI/DCS common toxicity criteria.

GM-CSF

Anticipated toxicities from GM-CSF administration in this dose range are expected to be mild based on previous experience. Potential toxicities include fever, chills, myalgias, arthralgias, nausea, vomiting, diarrhea, dyspnea, tachycardia, arrhythmias, elevation of liver function tests, elevation of BUN and creatinine. However, local skin reactions, such as erythema and induration, may be observed and will be carefully noted. Attempts will be made to maintain these patients as outpatients. For grade IV fever (not responsive to Indocin or Tylenol), or grade DI vomiting (unresponsive to therapy), GM-CSF will be held until toxicity is less than grade II and will be restarted at 50% of the original dose level for the rest of that weekly injection cycle and for subsequent cycles. For neurologic toxicity that affects daily function (unable to carry on simple routine duties, or grade II in the toxicity grading scale), hold treatment until symptoms resolve, then reduce GM-CSF by 50%. If symptoms persist, the adjuvant should be removed for subsequent immunizations. Patients with grade III neurotoxicity will be removed from the study.

For well-documented evidence of cardiac toxicity (i.e., grade DI, including evidence of ischemia or ventricular arrhythmia, but not supraventricular tachycardia or atrial fibrillation controlled by digoxin or calcium channel blocking agents), the adjuvant will be removed for subsequent immunizations.

Asymptomatic elevations in serum bilirubin and creatinine (not resulting in hyperkalemia) will be tolerated. For SGOT or SGPT >10× normal, GM-CSF will be held until values return to <5× normal, then resumed at 50% of the (3M-CSF dose for all remaining doses.

Fever and chills associated with vaccine administration and/or GM-CSF will be treated with TYLENOL and/or DEMEROL. The use of non-steroidal antiinflammatory drugs and/or steroids should be avoided. Should non-steroidals or steroids be required for unrelated medical conditions for a course exceeding 2 weeks, the patient will be taken off of the study.

Adverse Drug Reactions

All toxicities and adverse events will be recorded on the study flow sheet and appropriately graded as to severity and cause. Toxicities that are related to the underlying disease should be clearly differentiated from drug toxicities.

Adverse drug reactions related to chemotherapy will be submitted based on guidelines for commercial drugs.

Reports of adverse reactions to Id-KLH and GM-CSF will be made using the Division of Cancer Treatment Common Toxicity Criteria for reference according to the guidelines published by the DCT, NCI. These guidelines can be summarized as follows:

-   -   A. Report by telephone to IDB within 24 hours (301) 230-2330         -   1. All life-threatening events (grade 4, except for grade 4             myelosuppression) which may be due to administration of the             investigational drug(s),         -   2. All fatal events (grade 5),         -   3. All first occurrences of any previously unknown toxicity             (regardless of grade).     -   B. A written report should follow within 10 working days.     -   C. All adverse drug reactions will also be reported in writing         to the NCI Institutional Review Board within 10 working days.     -   D. All adverse drug reactions will also be reported to the FDA         in accordance with Federal regulations.     -   E. Data will be submitted at least every two weeks.

Study Parameters

During Chemotherapy

-   -   Weekly: CBC, diff. platelets; except day 14, i.e. CBC on day 0,         7, 21, and 28.     -   Beginning of each cycle: Chem 20, CXR, LAG follow-up (KUB), CT         scans (only after 4 cycles, then every 2 cycles).     -   Bilateral bone marrow aspirate and biopsy after four cycles and         every additional two cycles thereafter. Include 5 cc of aspirate         in PFH from each side for PCR analysis.

At Maximal Response to Chemotherapy

-   -   If residual disease is obvious, record measurements and perform         bone marrows as above.     -   For complete responders, complete restaging should be performed.         This should include all studies that were positive at initial         staging evaluation with the exception of repeat thoracotomy or         laparotomy. Bilateral bone marrows should be performed as above.

During Vaccine Therapy

-   -   If residual disease is obvious, record measurements and perform         bone marrows as above.     -   PT-PTT day 0     -   UA, β₂ microglobulin day 0 of each immunization.     -   Leukapheresis is performed on the day of initiation of vaccine         therapy (prior to the first cycle only) to obtain pre-vaccine         lymphocytes for storage. Five tiger top tubes are drawn at this         time to obtain serum for storage.     -   Two tiger top tubes and peripheral blood (60 cc in PFH) are         collected on day 0 of each monthly cycle, for preparation of         serum and lymphocytes, respectively.     -   Skin Biopsy is obtained near a planned immunization site on day         0 prior to the first cycle (baseline sample) and again on day 1,         2, or 3 of cycle 3 at an active site of erythema and/or         induration as close to the original biopsy site as possible.     -   DTH—Delayed type hypersensitivity test (DTH) to autologous         idiotype protein is performed during cycle 4 and again following         completion of the immunization regimen, i.e., during or after         cycle 5. The DTH-test is performed by intradermal injection of         0.5 mg of idiotype protein in 0.1-0.2 ml of NS. To ascertain the         specificity of a positive reaction, 0.5 mg of a heterologous         isotype matched Id-protein (from another patient on the same         study) in the same volume will be used as a negative control.         The control idiotypes used on these two occasions will be from         two different patients, also in the study, in order to minimize         the possibility of eliciting an immunologic response against a         particular irrelevant idiotype. A skin biopsy will also be         obtained at the site of the intradermal injection of idiotype         protein and at the control site, one to three days, after the         intradermal injections.     -   Fine needle aspiration or core biopsy (with or without CT         guidance) of any enlarged lymph node draining the vaccination         sites is performed to obtain lymphocytes for in vitro assays.

At Discontinuation of Vaccine

-   -   Restaging as described for Chemotherapy (see “At Maximal         Response to Chemotherapy,” above).     -   Bilateral bone marrow aspirates and biopsies at completion of         therapy and every six months for two years after completing         therapy and yearly thereafter.     -   10 cc of serum for storage and 60 cc of peripheral blood in PFH         is collected at completion of therapy and every three months for         a year.

Specimen Processing and Immunological Assays

Lymph Node Harvest/Biopsy

Each lymph node biopsy will be divided as follows: (a) one-third of the specimen will be sent in saline to the Hematopathology Section, Laboratory of Pathology, NIH. Biopsies are processed for routine histopathy and for immunophenotypic characterization, particularly with respect to monotypic heavy and light chain expression; and (b) two-thirds of the specimen is sent in sterile saline in a sterile container to Clinical Immunology Services, NCIFCRDC, where it is processed into a single-cell suspension and cryopreserved.

Blood and Bone Marrow Samples

All peripheral blood and bone marrow aspirate samples are sent in an expedited manner to Clinical Immunology Services, NCI-FCRDC. Tiger top tubes are spun down and serum divided into 1 ml aliquots for frozen storage. Peripheral blood mononuclear cells (PBMC) are isolated prior to freezing by Ficoll-hypaque centrifugation using standard protocols.

Assay for Serum Antibody

In a direct enzyme-linked immunosorbent assay (ELISA), preimmune and hyperimmune serum samples from each patient are diluted over wells of a microtiter plate that are coated with either autologous immunoglobulin idiotype or a panel of isotype-matched human tumor immunoglobulins of unrelated idiotype. Bound antibody is detected with horseradish peroxidase-goat antihuman light-chain antibodies directed against the light chain not present in the immunoglobulin idiotype (Caltag Laboratories, South San Francisco).

Assay for Idiotype-Specific Proliferative Response

Whenever feasible, fresh PBMC, isolated above, are used on the same day they are obtained. Stored frozen PBMC are available as a back-up. PBMC are washed and plated at a concentration of 4×10⁵ cells per well in Iscove's modified Dulbecco's medium (IMDM) with 1 percent human AB7 serum (IMDM-1 percent AB). KLH, autologous immunoglobulin idiotype, or a panel of isotype matched immunoglobulins of irrelevant idiotypes at concentrations of 0 to 100 μg per milliliter in IMDM-1 percent AB preparation are added in triplicate. After the cells are incubated for three days at 37° C. in an atmosphere containing 5 percent carbon dioxide, they are transferred to a preparation of IMDM and 5 percent fetal-calf serum containing recombinant interleukin-2 (30 U per milliliter). The plates are incubated for two days and pulsed for 16 to 20 hours with ³H-labeled thymidine (1 μCi per well). Data are expressed as mean (±SEM) counts per minute of [³H]thymidine incorporation.

Initial five-day cultures of PBMCs established as described above are expanded in IMDM-5 percent fetal-calf serum containing interleukin-2 (30 U per milliliter). Harvested cells are replaced in IMDM-1 percent AB containing autologous immunoglobulin idiotype and fresh irradiated (5000 R) autologous PBMCs (4×10⁵ cells per well) as antigen-presenting cells for five days, before pulsing with ³[H]thymidine.

Cytotoxicity Assays

The potential cytotoxicity of PBMC cultured with Id as above, or with irradiated fresh cryopreserved tumor cells, is assayed against either autologous lymphoblastoid cell lines (LBL) pulsed with Id or fresh cryopreserved tumor targets. Autologous LBL pulsed with soluble antigen have been used successfully as targets to detect gp 160-specific cytotoxic T-lymphocytes (20). Historically, the inability to establish long-term cultures of follicular lymphoma has hindered their availability as targets. However, two recent reports have described the use of fresh cryopreserved lymphoma cell targets, with levels of spontaneous incorporated radioisotope release in the acceptable range of <35% (21-22). Standard four hour ⁵¹Cr release, as well as 18-24 hour ¹¹¹In release assays are used.

Autologous LBL are prepared from pre-immune PBMC by the AIDS Monitoring Laboratory, NCI-FDRDC, using published methods.

Monitoring of T-Cell Receptor (TCR) Status

Pre-chemotherapy and pre- and postimmunization serum samples are assayed for TCR status by Western blot assay. Approximately 7×10⁶ purified T-cells from PBMC are lysed for 5 minutes at 4° C. in lysis buffer (25 mM Tris, pH 7.4 [Sigma Chemical Co., St Louis, Mo.], 300 mM NaCl, 0.05% Triton X-100, 1 mM Na orthovanadate, 10 μg/ml aprotinin, 10 μg/ml leupeptin, 10 mM nitrophenol-guanidine benzoate [NPGB] and 5 mM EDTA). The lysates are centrifuged at 12,000 rpm at 4° C. for 5 minutes and supernatant is removed with a micropipettor, making sure the nuclear pellet is not disturbed. A sample of the supernatant is then used to quantitate protein using the BCA protein assay (Pierce, Rockford, Ill.). The rest of the lysate is boiled with 3× reducing sample buffer for 5 minutes and placed on ice before its use in Western blot.

Varying concentrations of cellular lysate ranging between 1 and 30 μg are electrophoresed in 14% Tris-glycine gels (Novex Experimental Technology, CA) under reducing conditions and then transferred to Imobilon-p PVDF transfer membranes (Millipore Co., Bedford, Mass.). The membranes are incubated with a 5% solution of non-fat dried milk for one hour and then blotted for one hour at room temperature with anti-TCRζ anti-serum (Onco-Zeta 1, OncoTherapeutics, Cranbury, N.J.) at a 1:2000 dilution. The membranes are washed with TBS-T buffer [1 M Tris base, 5M NaCl, 0.1% Tween 20 (pH 7.5)] and incubated with anti-rabbit or anti-mouse Ig horseradish peroxidase (Amersham, Buckinghamshire, UK). After washing with TBS-T, the membranes are developed with the chemiluminescence kit ECL (Amersham, UK) for 1-5 minutes. X-OMAT AR film (Kodak Co., Rochester, N.Y.) is used to detect the chemiluminescence.

PCR Amplification of Rearranged bcl-2

Nested oligonucleotide amplification is performed at the MBR or mcr of the bcl-2/Ig_(H) hybrid gene using previously published methods (23). Briefly, samples containing 1 μg of genomic DNA are initially amplified for 25 cycles in a final volume of 50 μg containing 50 mmol/L KCl, 10 mmol/L Tris HCL, 2.25 mmol/L MgCl₂, 200 mmol/L oligonucleotide primers, 200 mmol/L each of dGTP, dCTP, dTTP and dATP, and 1.5 U Taq polymerase (Cetus, Emeryville, Calif.). Reamplification of an aliquot of product is performed for 30 cycles in a final volume of 50 μl using identical conditions to the original amplification, with oligonucleotide primers internal to the original primers. Aliquots of the final product are analyzed by gel electrophoresis in 4% agarose gels containing ethidium bromide and visualized under UV light. DNA is Southern blotted onto Zeta-probe blotting membrane (BioRad. Richmond, Calif.) and bcl-2-specific DNA is detected by hybridization with oligonucleotide probes radiolabeled with ³²P(ATP) using T4 polynucleotide kinase.

Removal of Patients from Protocol Therapy

Patients will be removed from protocol for any of the following reasons:

Unacceptable toxicity (as defined above).

The patient declines further therapy.

The patient experiences progressive lymphoma.

It is deemed in the best interest of the patient. In this instance,

-   -   The Principal Investigator should be notified.     -   The reasons for withdrawal should be noted in the flow sheet.

Response Criteria

Patients will be reevaluated for tumor response after every two cycles of chemotherapy using the following criteria:

Complete Response—disappearance of all clinical and laboratory (excluding PCR) signs and symptoms of active disease for a minimum of one month.

Partial Response—a 50% or greater reduction in the size of the lesions as defined by the sum of the products of the longest perpendicular diameters of all measured lesions lasting for a minimum of one month. No lesions may increase in size and no new lesions may appear.

Minimal Residual Response—a ≧90% partial response. For most patients in this category, this will mean ≦10% residual bone marrow involvement by lymphoma.

Progressive Disease—an increase of 25% or more in the sum of the products of the longest perpendicular diameters of all measured indicator lesions compared to the smallest previous measurement or the appearance of a new lesion.

Drug Formulation and Toxicity Data

Cyclophosphamide (CTX. Cytoxan)-NSC #26271

-   -   Source and Pharmacology—CTX is an alkylating agent, related to         nitrogen mustard, which is biochemically inert until it is         metabolized to its active components by the liver         phosphoramidases. It is non-phase-specific. The drug is excreted         exclusively by the kidney after parenteral administration.     -   Formulation and Stability—CTX is supplied as a 100, 200, 500,         1000 mg and a 2 gram lyophilized powder with 75 mg mannitol per         100 mg (anhydrous) cyclophosphamide. The vials are stored at         room temperature (59-86° F.) and reconstituted with sterile         water for injection to yield a final concentration of 20 mg/ml         as described in the package insert. Reconstituted         cyclophosphamide is stable for at least 6 days under         refrigeration and for 24 hours at room temperature.         Reconstituted drug and diluted solutions should be stored under         refrigeration.     -   Supplier—Commercially available.     -   Route of Administration—The cyclophosphamide used in this         regimen is given IV over 30 minutes and is diluted in 100 cc of         either D₅W or NSS.     -   Toxicity—Toxicities described with cyclophosphamide include         nausea, vomiting, myelosuppression, gonadal failure in both         males and females, alopecia, interstitial pneumonitis, pulmonary         fibrosis. hemorrhagic cystitis, cardiac events (cardiomyopathy),         syndrome of inappropriate antidiuretic hormone secretion (SIADH)         and rarely, anaphylaxis.

Prednisone (Deltasone. Meticorten, Liquid Pred) NSC#10023

-   -   Source and Pharmacology—Prednisone is the synthetic congener of         hydrocortisone, the natural adrenal hormone. It binds with         steroid receptors on the nuclear membrane, blocks mitosis, and         inhibits protein synthesis. It kills primarily during the         S-phase of the cell cycle. It is catabolized in the liver and         excreted in the urine. Peak blood levels occur within two hours         after oral intake. Plasma half-life is 3-6 hours. (Biologic         half-life is 12-30 hours.)

Cortisone 25 Hydrocortisone 20 Prednisone 5 Decadron 0.75 Equivalent strength in mg

-   -   Formulation and Stability—Available in 1, 2.5, 5, 10, 20 and 50         mg tablets; 5 mg/5 ml liquid.     -   Supplier—Prednisone is commercially available.     -   Route of Administration—PO; NOTE: May cause GI upset; take with         meals or snacks. Take in the morning prior to 9 a.m.     -   Toxicity—Toxicities described with prednisone include fluid and         electrolyte changes, edema, hypertension, hyperglycemia,         gastritis, osteoporosis, myopathy, behavioral and mood changes,         poor wound healing, and Cushing's syndrome (moon face, buffalo         hump, central obesity, acne, hirsutism and striae).

VP-16 (Etoposide. VePesid) NSC#141540

-   -   Source and Pharmacology—VP-16 is a semisynthetic derivative of         podophyllotoxin which inhibits topoisomerase II and functions as         mitotic inhibitor, but does not bind microtubules. Its main         effect appears to be in the S and G₂-phase of the cell cycle.         The mean terminal half-life is 11.5 hours, with a range of 3 to         15 hours. It is primarily excreted in the urine.     -   Formulation and Stability—VP-16 is supplied in vials containing         either 100 or 500 mg of etoposide (20 mg/ml) in a polyethylene         vehicle. VP-16 is diluted in either 500 cc of 5% dextrose or         0.9% Sodium Chloride Injection. Diluted solutions         (concentrations of 0.2, 0.4 mg/ml and 1 mg/ml) are stable for         96, 48 hours and 2 hours, respectively at room temperature under         normal room fluorescent light in both glass and plastic         containers. Do not refrigerate etoposide-containing solutions.     -   Supplier—VP-16 is commercially available.     -   Route of Administration—Etoposide is administered as an IV         infusion over 60 minutes.     -   Toxicity—Toxicities described with etoposide administration         include myelosuppression (neutropenia), nausea, vomiting,         mucositis, allergic reactions characterized by anaphylactic         symptoms and hypotension and alopecia.

Doxorubricin (Adriamycin) NSC #123127

-   -   Source and Pharmacology—Doxorubicin is an anthracycline         antibiotic isolated from cultures of Streptomyces peucetius. It         binds to DNA and inhibits nucleic acid synthesis, with its major         lethal effect occurring during the S-phase of the cell cycle.         Since it is primarily excreted by the liver, any liver         impairment may enhance toxicity. Some of the drug has a very         short α T ½ of <20 minutes and a β ½ of 17 hours. Animal studies         indicate cytotoxic levels persist in tissue for as long as 24         hours. Biliary excretion also is a source of elimination for         Doxorubicin; therefore, patients with         hyperbilirubinemia/cholestasis caused by something other than         lymphoma should have dosage modification.     -   Formulation and stability—Doxorubicin is available as a         freeze-dried powder in 10, 50 and 150 mg vials. The drug is         stored at room temperature, protected from light, and is         reconstituted with sodium chloride 0.9% (NSS) to yield a final         concentration of 5 mg/ml. The reconstituted solution is stable         for 7 days at room temperature (1 5-30° C.) or if stored under         refrigeration (2-8° C.).     -   Supplier—Doxorubicin is commercially available.     -   Route of Administration—Doxorubicin is given as a slow IV         injection over 5-7 minutes through an established line with a         free flowing IV.     -   Special precautions: Avoid extravasation and local contact with         skin or conjunctiva.     -   Toxicity—Toxicities described with doxorubicin administration         include myelosuppression, nausea, vomiting, mucositis,         stomatitis, alopecia. diarrhea, facial flushing, dose-related         congestive cardiomopathy, arrhythmias, vein streaking         (hypersensitivity reaction), radiation-recall dermatitis, local         cellulitis, vesication and tissue necrosis upon extravasation         (SQ and dermal necrosis).

ID-KLH Vaccine

-   -   Source—Idiotype protein from the individual B cell lymphomas is         obtained from tissue culture, purified, and covalently coupled         to keyhole limpet hemocyanin (KLH) as previously described. Each         batch is produced according to Good Manufacturing Practices         standards and tested for sterility, endotoxin contamination, and         general safety prior to its use in any patient. The preparation         and quality control/quality assurance testing of the Id-KLH         conjugate is performed by TSI Washington under CRB contract. The         IND for the Id-KLH vaccine will be held by the Drug Regulatory         Affairs Section, CTEP.     -   How supplied—Formulated product for subcutaneous administration         contains 0.5 mg of Id and KLH each per ml of normal saline.         Id-KLH is supplied as a 1 ml vial.     -   Storage—Prior to administration, Id-KLH is stored at −20° C.     -   Administration—After thawing and gentle agitation, the vial         contents are drawn up using an 18-gauge needle on a syringe.         After the entire contents have been drawn up, the 18-gauge         needle is replaced by a 25-gauge needle for injection. This         procedure is important to ensure that all particulates (normal         components of this vaccine) are obtained from the vial.     -   Toxicity—Toxicities described with Id-KLH vaccine administration         include local site reactions (erythema, induration, swelling and         tenderness), fever, chills, rash, myalgias and arthralgias. Mild         elevations in creatinine phosphokinase (CPK) have been observed.

GM-CSF (Sargramostim: NSC #613795; BB-IND 2632

-   -   Source and Pharmacology—The GM-CSF used in this study is         glycosylated, recombinant human GM-CSF. This GM-CSF is an         altered form of the native molecule; the position 23 arginine         has been replaced with a leucine to facilitate expression of the         protein in yeast (Saccharomyces cerevisiae).     -   Formulation and Stability—The GM-CSF is formulated as a white         lyophilized cake and is provided in vials containing 500 μg of         the GM-CSF protein as well as 10.0 mg of sucrose, 40.0 mg of         mannitol, and 1.2 mg of Tris (Trimethamine).     -   To prepare a vial of GM-CSF for direct subcutaneous use,         aseptically inject 1.0 ml of Sterile Water for Injection, USP,         into the vial to dissolve the lyophilized cake. The diluent         should be directed against the side of the vial to avoid excess         foaming. Avoid vigorous agitation of the vial; do not shake.         This yields a solution containing 500 μg/ml. The unreconstituted         material should be kept refrigerated at 2-8° C. and is stable         for at least eighteen months. Once reconstituted, the solution         is stable for at least 24 hours at 2-8° C. or at 18-25° C.         Because the product does not contain a preservative, vials         should be treated as unit-dose containers; reconstituted         solution should be held at 2-8° C. and discarded after no more         than six hours. Do not freeze GM-CSF.

Supplier. Manufactured by Immunex.

-   -   Route of Administration—The appropriate total dose is withdrawn         into and administered from a plastic tuberculin syringe. The         GM-CSF is injected subcutaneously as close as possible to the         Id-KLH injection site. All GM-CSF doses for each patient are         administered by the nursing staff in the outpatient unit.     -   Toxicity—Toxicities described in patients receiving GM-CSF         include: fever, chills, diaphoresis, myalgias, fatigue, malaise,         headache, dizziness, dyspnea, bronchospasm, pleural effusion,         anorexia, indigestion, nausea, vomiting, diarrhea, injection         site tenderness, urticaria, rash, pruritus, hypersensitivity         reaction, bone pain, thromboembolic events, phlebitis,         hypotension, peripheral edema, leukocytosis, thrombocytosis or         thrombocytopenia, hepatic enzyme abnormalities, and bilirubin         elevation. The first administration of GM-CSF has provoked a         syndrome of dyspnea and hypotension within two hours after         GM-CSF injection in a single patient receiving yeast-derived         GM-CSF; this type of reaction has more frequently been observed         in patients receiving GM-CSF produced in E. coli. One report of         a vascular leak-like syndrome occurring after autologous bone         marrow transplant in a patient receiving continuous IV infusion         of GM-CSF has been recorded.

Unconjugated Lymphoma Immunoglobulin Idiotype (for Intradermal Skin Testing) NSC#684151

-   -   Source—The patient-specific purified idiotype protein,         previously produced according to GMP standards as described         above, is vialed as a separate product by TSI Washington         Laboratories and will be supplied by CTEP, DCT, NCI. This vialed         product is tested separately for sterility, endotoxin, and         mycoplasma, according to IND specifications previously discussed         with the FDA.     -   Each vial of patient-specific unconjugated idiotype will be         labeled to include the following information:         -   Purified sterile immunoglobulin idiotype patient-specific             lot         -   final volume and concentration of product         -   patient-specific immunoglobulin subtype         -   storage conditions         -   fill date         -   patient identification (first name/last initial)     -   How Supplied—This product is available as a solution containing         0.2-0.3 ml of unconjugated idiotype diluted in sodium chloride         0.9%. The solution is contained inside a sterile vial. The final         solution contains 0.5 mg of patient-specific immunoglobulin         idiotype protein. Intact vials are stored at −20° C.     -   Toxicity—The toxicities associated with administration of         unconjugated Id protein are anticipated to be identical to those         described with the Id-KLH vaccine.         -   The safety issues regarding the injection of heterologous             idiotype protein isolated from other patients' B-cell tumors             have already been fully addressed in CRB #9407 (NCI             T94-0085; Active immunization of Healthy Sibling Marrow             Transplant Donors With Myeloma-derived Idiotype) and are             felt to be minimal, because of the highly purified nature of             the protein.         -   Briefly, an immune response of any consequence to the             isotype matched idiotype used as a negative control during             the second skin test is not likely, based on:         -   1. The isotype matched idiotype will only be administered             once and is not conjugated to a carrier protein. These             minimize the chance of eliciting a sustained immune response             to the protein.         -   2. Any immune response specifically directed against the             idiotype (i.e., variable region) on the control idiotype             protein is not likely to cross-react with host cells and is             therefore not likely to be of any consequence.         -   3. An autoimmune response against constant region or             allotype determinants shared between the idiotype of the             patient's own tumor and that of the control idiotype tumor             is theoretically possible. However no evidence of such             autoimmune responses have been observed either in vivo or in             vitro during the course of immunization of sibling bone             marrow transplant donors with purified myeloma protein.         -   Furthermore, a safety precedent exists for immunizing             patients with material derived from tumor cells from other             patients. For example, in attempting to develop immune             responses against metastatic melanomas, patients were             immunized with 1) intact melanoma cells; 2) shed antigens             fractionated by detergent treatment and             ultracentrifugation; 3) melanoma cells infected with             vaccinia virus and melanoma cells freeze thawed and             mechanically disrupted, all using a pool of allogeneic             melanoma cell lines (24-28).

Bactrim will be supplied by the Clinical Center.

Filgrastim (G-CSF)/Neupogen

-   -   Source and Pharmacology—The G-CSF to be used in this study is         the recombinant methionyl human granulocyte-colony stimulating         factor (r-methi-HuG-CSF). G-CSF is a hematopoietic growth factor         with effects on both immature bone marrow progenitors and mature         myeloid cells. It acts by supporting growth of human bone marrow         derived colony forming units and enhancing neutrophil growth and         proliferation.     -   Formulation and Stability—The G-CSF is formulated as a clear,         sterile solution and is provided in vials at a final         concentration of 300 mcg/ml. The commercial vials are available         in 300 and 480 mcg sizes. The intact vials are stored under         refrigeration (2-8° C.) prior to use and must not be frozen and         are stable at this temperature for at least one year.     -   Supplier—Manufactured by Amgen; supplied by the Clinical Center.     -   Route of Administration—The appropriate total dose is withdrawn         into and administered from a plastic tuberculin syringe. The         G-CSF is injected as a subcutaneous injection. The patient or         other care-giver is instructed on proper injection technique.     -   Toxicities—Toxicities described with G-CSF include: transient         bone pain (sternal/pelvic) myalgias, fatigue, mild elevations in         uric acid, LDH and alkaline phosphate, fluid retention,         transient hypotension, local inflammation at injection site,         rarely cutaneous vasculitis, rarely pericardial effusion and         rare anaphylactic reactions with first dose.

Statistical Considerations

Statistical issues to be addressed include identification of significant endpoints, sample size determination, power considerations, stratification, randomization and design.

The design of this study is viewed primarily within the framework of a Single Arm Phase II trial. However, as the purpose is also to investigate possible differences between GM-CSF doses as adjuvants, it incorporates design elements characteristic of a Multiple Arm Phase II or a randomized Phase III trial. Statistical methods that are appropriate to both single and double arm designs are described. Patients receive combination chemotherapy to best response followed by Id-KLH combined with GM-CSF. Several outcome measures (endpoints) are evaluated.

in order to meet the objectives of this study. They include:

1) The clinical complete response rate (in contradistinction to the molecular or PCR response rate) of all patients to ProMACE—a percentage indicated by the disappearance of all clinical and laboratory signs and symptoms of active disease, excluding PCR, for a minimum of one month.

2) The Polymerase Chain Reaction (PCR) response rate (molecular—complete response rate)—the percentage of patients who, having achieved a clinical complete response still remain PCR (+) at the end of chemotherapy, and who then become PCR (−) with the administration of immunotherapy.

3) Disease Free Survival Rate—computed by Kaplan-Meier curves and related survival measures.

The PCR response rate is taken as the primary outcome variable of interest to ascertain the following: (1) to determine the ability of Id immunization to eradicate bcl-2 positive tumor cells from the bone marrow and; (2) to identify the more biologically active of the two doses of GM-CSF. In this endeavor, the plan is to accrue 42 patients. It is estimated that approximately 38 (90%) of these patients will be bcl-2 (+) and thus evaluable for molecular response rate. The other four patients may still be evaluable for a molecular response rate based on Ig gene amplification using allele-specific (CDR3) primers by PCR. From previous experience with ProMACE-based regimens, it is estimated that 32 (85%) of these patients will achieve either a complete response (complete clinical response, CCR) or a partial response in which a >90% partial remission has been obtained (high partial response, HPR). The accuracy of these estimates are of some interest. For the 42 (90%) patients anticipated to be bcl-2 (+), lower and upper 95% confidence intervals are 77% and 96%. For the 38 (85%) patients anticipated to achieve either a complete clinical response or a high partial response, the lower and upper confidence intervals are 70% and 93%.

Patients are stratified on the basis of their ProMACE treatment performance as either a complete clinical responder (CCR) or as a high partial responder (HPR). It is not known exactly what percentage of these 32 patients will be CCRs and what percentage will be HPR'S. Hence a block size of four (4) is used in the randomization scheme to assure a reasonably balanced allocation to each dose group. Given the patients allocation stratum, he (she) is randomly assigned to one of the adjuvant groups according to the envelope method (29). Specifically, a block of four assignments is placed in four separate envelopes. The block of four is placed in one of the two allocation strata, say CCR. Another block of four is placed in the other allocation strata, say CCR. Another block of four is placed in the other allocation stratum, HPR. When a patient is to be randomized, a call is made to the biostatistician who, after being informed of the patients status as either a CCR or an HPR, randomly draws an envelope from the appropriate stratum to determine the patients dose group assignment. After the four envelopes pertinent to a particular stratum have been exhausted, the next batch of four envelopes is made available for use. This procedure is continued until a total of 32 patients have been assigned to the two dose groups.

For example, it is estimated that 50-80 percent of pathological complete responders will fall into the CCR category. If 75% of 32, or 24 patients were to be classified as CCRs, six blocks of four envelopes would be required to randomly assign 12 patients to cohort 1 and 12 patients to cohort 2. A similar procedure would occur concurrently with the 8 patients classified as HPRs. Two blocks of four envelopes would be required to randomly assign 4 patients to cohort 1 and 4 patients to cohort 2. At no time could the number of patients in each dose group differ by more than four.

At the time of data analysis, approximately 16 subjects will comprise each dose group and a test for the difference in PCR response rates between the two groups will be conducted. By hypothesis, neither dose group is predicted to have a higher PCR response rate than the other; hence, a two-tailed test is appropriate. Power calculations show that, with the groups limited to 16 patients, the difference in PCR response rates will have to be large (30, 31). For example, to detect a difference at the α=0.05 level of significance with power (1−β) equal to 80%, the response rates must differ by 55%; with power equal to 50%, the response rates must differ by 50%. In the event that no significant difference is detected, the subjects will be pooled and the overall PCR response rate will be assessed. With a total of 32 CCRs and HPRs treated with vaccine, the width of a two-tailed 95% confidence interval for a response rate of 50% will not exceed 17 percentage points. If the actual response rate is higher or lower than 50%, the confidence interval will be smaller.

Disease-free survival distributions are estimated by the Kaplan-Meier (product-limit) method and dose groups are compared using the log rank test. If no dose group differences are detected, the subjects from both groups are pooled and the Kaplan-Meier estimate of the survivorship function and related functions are evaluated. If suggested by the data analysis, parametric distributions (e.g., Weibull, log-normal) are fit as well (32, 33).

Research ethics: Subjects from [both genders and] all racial/ethnic groups are eligible for this study if they meet the eligibility criteria outlined above. To date, there is not information that suggests that differences in grud metabolism or disease response would be expected in one group compared to another. Efforts are made to extend accrual to a representative population, but in this preliminary study, a balance must be struck between patient safety considerations and limitations on the number of individuals exposed to potentially toxic and/or ineffective treatments on the one hand and the need to explore gender and ethnic aspects of clinical research on the other hand. If differences in outcome that correlate to gender or to ethnic identity are noted, accrual can be expanded or a follow-up study can be written to investigate those differences more fully. Alternatively, substantial scientific data exist demonstrating that there is no significant difference in outcome between genders or various ethnic groups.

Records to be Kept and Quality Assurance

Consent form: The original signed informed consent documents will be kept with the patient's other study documentation (e.g., the research chart). A copy of the informed consent document will also be retained by the Data Management Section.

The Clinical Coordinator, Data Management Section, will ascertain the dates of the IRB approvals before registering the first patient.

It is understood that the disclosed invention is not limited to the particular methodology, protocols, and reagents described as these may vary. It is also to be understood that the terminology used herein is for the purpose of describing particular embodiments only, and is not intended to limit the scope of the present invention which will be limited only by the appended claims.

It must be noted that as used herein and in the appended claims, the singular forms “a”, “an”, and “the” include plural reference unless the context clearly dictates otherwise. Thus, for example, reference to “a host cell” includes a plurality of such host cells, reference to “the antibody” is a reference to one or more antibodies and equivalents thereof known to those skilled in the art, and so forth.

Unless defined otherwise, all technical and scientific terms used herein have the same meanings as commonly understood by one of skill in the art to which the disclosed invention belongs. Although any methods and materials similar or equivalent to those described herein can be used in the practice or testing of the present invention, the preferred methods, devices, and materials are as described. Publications cited herein and the material for which they are cited are specifically incorporated by reference. Nothing herein is to be construed as an admission that the invention is not entitled to antedate such disclosure by virtue of prior invention.

Those skilled in the art will recognize, or be able to ascertain using no more than routine experimentation, many equivalents to the specific embodiments of the invention described herein. Such equivalents are intended to be encompassed by the following claims.

REFERENCES

-   1. Stevenson G T, Stevenson F K. Antibody to molecularly defined     antigen confined to a tumor cell surface. Nature, 1975, 254:714-6. -   2. Stevenson G T, Elliott E V, Stevenson F K, Idiotypic determinants     on the surface Immunoglobulin of neoplastic lymphocytes: a     therapeutic target. Fed Proc, 1977, 36:2268-71. -   3. Miller P A, Maloney D G, Wamke R, Levy R. Treatment of B cell     lymphoma with monoclonal anti-idiotype antibody. N Engl J Med, 1982,     306; 517-22. -   4. Sirisinha S, Eisen H N. Autoimmune-like antibodies to the     ligand-binding sites of myeloma proteins. Proc Natl Acad Sci USA,     1971, 68:3130-5. -   5. Jorgensen T, Gaudemack G, Hannestad K. Immunization with the     light chain and the VL domain of the isologous myeloma protein 315     inhibits growth of mouse plasmacytoma MOPC-315. Scand J Immunol,     1980, 11:29-35. -   6. Daley M J, Gebel H M, Lynch R G. Idiotype-specific     transplantation resistance to MOPC-315: Abrogation by     post-immunization thymectomy. J Immunol, 1978, 120:1620-4. -   7. Bridges S H. Participation of the humoral immune system in the     myeloma-specific transplantation resistance. J Immunol, 1978,     121:479-83, -   8. Freedman P M, Autry J R, Tokuda S, Williams R C, Jr. Tumor     immunity induced by preimmunization with BALB/c mouse myeloma     protein. J Natl Cancer Inst. 1976, 56:735-740. -   9. Sugai S, Palmer D W, Taial N. Witz I F Protective and cellular     immune responses to idiotypic determinants on cells from a     spontaneous lymphoma of NZB/NZWP1 mice. J Exp Med, 1974,     140:1547-58. -   10. Stevenson F K, Gordon I. Immunization with idiotypic     immunoglobulin protects against development of B lymphocytic     leukemia, but emerging tumor cells can evade antibody attack by     modulation. J Immunol, 1983, 130:970-973. -   11. George A J T, Tutt A L, Stevenson F K. Anti-idiotypic mechanisms     involved in the suppression of a mouse B cell lymphoma, BCL. J     Immunol, 1987, 138:628-634. -   12. Kaminski M S, Kitamura K, Maloney D G, Levy R. Idiotype     vaccination against murine 13 cell lymphoma. Inhibition of tumor     immunity by free idiotype protein. J Immunol, 1987, 138:1289-1296. -   13. Kwak L W, Campbell M J, Zelonetz A D, Levy R. Combined syngeneic     bone marrow transplantation and immunotherapy of a murine B-cell     lymphoma: Active immunization with tumor-derived idiotypic     immunoglobulin. Blood, 1990, 76:2411-2417. -   14. Campbell M J, Esserman L. Byars N E, Allison A C, Levy R.     Development of a new therapeutic approach to B cell malignancy: the     induction of immunity by the host against cell surface receptor on     the tumor. Int Rev immunol, 1989, 4:251-70. -   15. Kwak L W, Campbell M J, Czervwinski D K, Hart S, Miller R A,     Levy R. Induction of immune responses in patients with B cell     lymphoma against the surface immunoglobulin idiotype expressed by     their tumors. N Engl J Med, 1992, 327:1209-1215. -   16. Longo D L-Young R C, DeVita V T. What is so good about the “good     prognosis” lymphoma? In Williams C G, Whithouse JMA (eds): Recent     Advances in Clinical Oncol Edinburgh, Churchill-Livingstone, pp.     223-231,1982. -   17. Portlock C S. “Good risk” non-Hodgkin's lymphomas. Approaches to     management. Sem Hematol, 1980.20:25-34. -   18. Portlock C S, Rosenberg S A. No initial therapy for stage III     and IV non-Hodgldn's lymphomas of favorable histologic types. Ann     Intern Med, 1979, 90:10-13. -   19. Horning S J, Rosenberg S A. The natural history of initially     untreated low-grade non-Hodgkin's lymphomas. N Engl J Med, 1984,     311:147-51. -   20. Orentas R J. Hildreth J E K, Obah E, Polydefkis M. Smith G E,     Clements M L, Siliciano R F. Induction of CD4+human cytolytic T     cells specific for HIV-infected cells by a gp 160 subunit vaccine.     Science, 1990, 248:1234-6. -   21. Schwartzentruber D J, Stetter-Stevenson M. Rosenberg S A,     Topalian S L. Tumor infiltrating lymphocytes derived from select     B-cell lymphomas secrete granulocyte-macrophage colony-stimulating     factor and tumor necrosis factor-α in response to autologous tumor     stimulation. Blood, 1993, 82:1204-11. -   22. Schlegal P G. Schmidt-Wolf G, Schmidt-Wolf G H, Kwak L W, Blume     K G, Chao N J. Lymphokine-activated killer cell activity against     autologous lymphoma cells following bone marrow transplantation.     Cancer Res. 1993, in press. -   23. Gribben J O, Freedman A S, Neuberg D, Roy D C, Blake K W, Woo S     D, Grossard M L, Rabinow S N, Coral F, Freeman G I, Ritz I, Nadler     L M. Immunologic purging of marrow assessed by PCR before autologous     bone marrow transplantation for B-cell lymphoma. N Engl J Med, 1991,     325:1525. -   24. Morton D L, et al. Annals New York Academy of Sciences.     Polyvalent melanoma vaccine improves survival of patients with     metastatic melanoma. 120; 1993. -   25. Bystryn J C. Annals New York Academy of Sciences. Immunogenicity     and clinical activity of a polyvalent melanoma antigen vaccine     prepared from shed antigens. 190; 1993. -   26. Wallack M K. Annals New York Academy of Sciences. Clinical     trials with VMo for melanoma. 178; 1993. -   27. Hershey P. Annals New York Academy of Sciences. Evaluation of     vaccinia viral lysates as therapeutic vaccines in the treatment of     melanoma. 167; 1993. -   28. Mitchell M S, et al. Annals New York Academy of Sciences. Active     specific immunotherapy of melanoma with allogeneic cell lysates.     153; 1993. -   29. Lesser M L. Design and implementation of clinical trials. In:     Statistics in Medical Research—Methods and Issues with Applications     in Cancer Research. Ed: Mike V and Stanley K F, New York, Wiley.     1982. -   30. Gehan E A, Schneiderman M A: Experimental Design of Clinical     Trials, in Holland J F and Frei E, III, eds. Cancer Medicine (2nd     ed.). Lea and Febinger, Philadelphia, 531-553,1982. -   31. Gail M, Gart J J: The Determination of Sample Sizes for Use with     the Exact Conditional Test in 2×2 Comparative Trials. Biometrics,     29, 441-448, 1973. -   32. Lee E T: Statistical Methods for Survival Data Analysis, Wiley,     New York, 1992. -   33. Kalbfleisch J D, Prentice R L: The Statistical Analysis of     Failure Time Data, New York, Wiley, 1980. -   34. Current protocols in immunology. J. E. Coligan, A. D.     Kruisbeek. D. H. Margulies, E. M. Sgevach and W. Strober, Eds. (J.     Wiley & Sons, Inc., New York, 1994), p. -   35. B. A. Ben, et al, J. Immunol. 158, 5927 (1997). -   36. Bergmanm Y., J. Haimovich, Characterization of a     carcinogen-induced murine B lymphocyte cell line of C3H/eb     origin. J. Immunol. (1977). 7: 413 -   37. Kwak et al. 1991. Transfer of specific immunity to B-cell     lymphoma with syngeneic bone marrow in mice. Blood 78:2768-2772. -   38. E-Blasi, et al. Nature 318, 667 (1985). -   39. R. Bonecchi, et al. J. Exp. Med. 187,129 (1998). -   40. J. Buchner, I. Pastan, U. Binkmann, Anal. Biochem. 205, 263     (1992). -   41. E. C. Butcher, Cell 67,1033 (1991). -   42. M. J. Campbell, et al, J. Immunol. 139. 2825 (1987). -   43. M. J. Campbell, L. Esserman. N. E. Byars, A. C. Alison, R. Levy,     Idiotype vaccination against murine B cell lymphoma. Humoral and     cellular requirements for the full expression of antitumor     immunity, J. Immunol. (1998) 145(3):1029-1036. -   44. H. L. Davis et al. Vaccine 15, 849 (1997). -   45. D. Dilloo et al. Nature Medicine 2, 1090 (1998). -   46. R. J. Dyke, H. McBride, A. J. George, T. J. Hamblin, F. K.     Stevenson, Cell Immunol 132, 70 (1991). -   47. W. J. Fairbrother, N-J-Skelton, Chemoattractant ligands and     their receptors., R. Horuk, Ed. (CRC, Boca Raton, NY, London, Tokyo,     1996), p. 55. -   48. A. Haelens, et al. Immunobiology 195, 499 (1996). -   49. I. Hakim, S. Levy, R. Levy, J. Immunol 157, 5503 (1996). -   50. J. S. Huston, H. Oppermann, inventors, Targeted multifunctional     proteins. USA. wo88 09344. (198). -   51. K. J. Kim, L. C. Kanellopoulos, R. M. Merwin, D. H. Sachs, R.     Asofsky, J. Immunol. 122, 549 (1979). -   52. L. W. Kwak et al. N. Engl. J. Med. 327,1209 (1992). -   53. L. W. Kwak, et al. Lancet 345, 1016 (1995). -   54. L. W. Kwak, H. A. Young, R. W. Pennington, S. D. Weeks, Proc.     Natl. Acad. Sci. U.S.A. 93, 10972 (1996). -   55. M. Loetscher et al., J. Exp. Med. 184, 963 (1995). -   56. P. Loetscher, M. Seitz, L. I. Clark, M. Baggiolini, B. Moser, J.     Immunol. 156, 322 (1996). -   57. A. D. Luster, P. Leder, J. Exp. Med. 178, 1057 (1993). -   58. A. D. Luster, N. Eng. J. Med, 338, 436 (1998). -   59. B. J, Rollins, Blood 90, 909 (1997). -   60. Y. Sato et al. Science 273, 352 (1996). -   61. J. M. Schroder, J. Invest. Dematol. 105,20S (1995). -   62. R. Salary et al, J. Biol. Chem. 272, 9617 (1997). -   63. M. B. Spellerberg et al., J. Immunol. 159, 1885 (1997). -   64. F. K. Stevenson et al., Immunol. Rev. 146. 211 (1996). -   65. R. M. Strieter et al., J. Biol. Chem., 270, 27348 (1995). -   66. C. J. Talpas, D. A. Walz, L. Lee, Biochim. Biophys. Acta 1078,     208 (1991). -   67. Y. Tanaka, D. H. Adams, S. Shaw, Immunol Today 14,111 (1993) -   68. G. J. Weiner, H. M. Liu, I. E. Wooldridge, C. E. Dahle, A. M.     Krieg, Proc. Nat. Acad. Sci. U.S.A. 94,10833 (1997) -   69. C. Winkler, et al, Science 279, 389 (1998). -   70. M, Yokoyama, D. P. Hassett, J. Mang, J. L. Whitton. Vaccine, 15,     553 (1997). -   71. Finn et al., 1995. Immunological Reviews 145:61-88; “Partially     purified tumor antigen vaccines” In: Biologic Therapy of Cancer:     Principles and Practice, 2nd ed. Edited by DeVita et al., J.B.     Lippincott Co., 1995). -   72. Old, L. J. “Cancer immunology: The search for specificity,” GHA     Clowes Memorial Lecture. Cancer Res. 41:361-375, 1981. -   73. Livingston, P. In: Biologic Therapy of Cancer: Principles and     Practice, 2nd ed. Edited by DeVita et al., J.B. Lippincott Co.,     1995. -   74. Harlow & Lane, Antibodies, A Laboratory Manual, Cold Spring     Harbor Laboratory, Cold Spring Harbor, N.Y., 1988. -   75. Baggioni, M., et al., 1994. IL-8 and related chemotactic     cytokines—CXC and CC chemokines. Adv. Immunol. 55:97-179. -   76. Garcia-Zepeda, E. A., et al., 1996. Human monocyte     chemoattractant protein (MCP)-4 is a novel chemokine with activities     on monocytes, eosinophils and basophils induced in allergic and     nonallergic inflammation that signals through the CC chemokine     receptors (CCR)-2 and -3. J. Immunol. 157:5613-5626. -   77. Clark-Lewis et al., 1991. Structure-activity relationship of     IL-8 determined using chemically synthesized analogs: critical role     of NH₂-terminal residues and evidence for uncoupling neutrophil     chemotaxis, exocytosis and receptor binding. J. Biol. Chem.     266:128-134. -   78. Weber, M., et al., 1996. Deletion of the NH₂-terminal residue     converts MCP-1 from an activator of basophil mediator release to an     eosinophil chemoattractant. J. Exp. Med. 183:681-685. -   79. The Oncogene Handbook, T. Curran, E. P. Reddy, and A. Salka     (ed.), Elsevier Science Publishers, The Netherlands (1988). -   80. Dayhoff et al., in Atlas of Protein Sequence and Structure 1978,     Nat'l Biomed. Res. Found., Washington, D.C. -   81. Sambrook et al., Molecular Cloning: A Laboratory Manual, 2d.     edition, Cold Spring Harbor Laboratory, Cold Spring Harbor, N.Y.,     1989. -   82. Brake et al., “Alpha-factor-directed synthesis and secretion of     mature foreign proteins in Saccharomyces cerevisiae,” PNAS     82:4642-4646, 1984. -   83. U.S. Pat. No. 4,704,362. -   84. Remington's Pharmaceutical Sciences (Martin, E. W., ed., latest     edition, Mack Publishing Co., Easton, Pa.). -   85. Harlow and Lane, Antibodies, A Laboratory Manual, Cold Spring     Harbor Laboratory, Cold Spring Harbor, N.Y., 1988). -   86. “Immunologic Studies in Humans,” Current Protocols in     Immunology, J. E. Coligan et al., eds. John Wiley & Sons, New York,     1991. -   87. Yamamoto et al., “Highly sensitive qualitative and quantitative     detection of reverse transcriptase activity: optimization,     validation and comparative analysis of other detection systems.” J.     Virol. Meth, 61:135-143, 1996. -   88. Kageyama, S. et al., “An improved method for the detection of     HIV antigen in the blood of carriers,” J. Viral. Meth. 22:125-131,     1988. -   89. Ho, D. D. et al., “Quantitation of human immunodeficiency virus     type 1 in the blood of infected persons,” N. Eng. J. Med.     321:1621-1625, 1988. -   90. Piatak, M. et al., “High levels of HIV-1 in plasma during all     stages of infection determined by competitive PCR,” Science     259:1749-1754, 1993. -   91. Mulder, J. et al., “Rapid and simple PCR assay for quantitation     of human immunodeficiency virus type 1 RNA in plasma: Application to     acute retroviral infection,” J. Clin. Microbiol. 32:292-300, 1994. -   92. Amon, R. (Ed.) Synthetic Vaccines 1:83-92, CRC Press, Inc., Boca     Raton, Fla., 1987. -   93. Willis et al., Gene 128:79-83, 1993. -   94. Jellis et al., Gene 137:63-68, 1993. -   95. Barbas et al., PNAS 89:4457-4461, 1992. -   96. Pastan et al. “A retrovirus carrying an MDR1 cDNA confers     multidrug resistance and polarized expression of P-glycoprotein in     MDCK cells.” Proc. Nat. Acad. Sci. 85; 4486 (1988). -   97. Miller et al. “Redesign of retrovirus packaging cell lines to     avoid recombination leading to helper virus production.” Mol. Cell.     Biol. 6:2895 (1986). -   98. Mitani et al. “Transduction of human bone marrow by adenoviral     vector.” Human Gene Therapy 5:941-948 (1994)). -   99. Goodman et al. “Recombinant adeno-associated virus-mediated gene     transfer into hematopoietic progenitor cells.” Blood 84:1492-1500     (1994)) -   100. Naidini et al. “In vivo gene delivery and stable transduction     of nondividing cells by a lentiviral vector.” Science 272:263-267     (1996)) -   101. Agrawal et al. “Cell-cycle kinetics and VSV-G pseudotyped     retrovirus mediated gene transfer in blood-derived CD34⁺ cells.”     Exp. Hematol. 24:738-747 (1996)). -   102. Schwarzenberger et al. “Targeted gene transfer to human     hematopoietic progenitor cell lines through the c-kit receptor.”     Blood 87:472-478 (1996)). -   103. Fields, et al. (1990) Virology, Raven Press, New York). -   104. Crystal, R. G. 1997. Phase I study of direct administration of     a replication deficient adenovirus vector containing E. coli     cytosine deaminase gene to metastatic colon carcinoma of the liver     in association with the oral administration of the pro-drug     5-fluorocytosine. Human Gene Therapy 8:985-1001. -   105. Alvarez, R. D. and D. T. Curiel, 1997. A phase I study of     recombinant adenovirus vector-mediated delivery of an anti-erbB-2     single chain (sFv) antibody gene from previously treated ovarian and     extraovarian cancer patients. Hum. Gene Ther. 8:229-242. -   106. Bergman, Y. & Haimovich, 3. Characterization of a     carcinogen-induced murine B lymphocyte cell line of C3H/eB origin.     Eur. J. Immunol. 7, 413-417,1977. -   107. Kim, K. J., Kanelloupolos-Langevin, C. Merwin, R. M.,     Sachs, D. H. & Asofsky, R. Establishment and characterization of     BALM lymphoma lines with B cell properties. J. Immunol. 122,     549-554, 1979. -   108. Huston, I S., Levinson, D., Mudgett-Hunter, M., Tai, M. S.,     Novotny, J., Margolies, M. N., Ridge, R. I., Bruccoleri, R. E.,     Haber, E., Crea R., & Opperman, H. Protein engineering of antibody     binding sites: Recovery of specific activity in an anti-digoxin     single-chain Fv analogue produced in Escherichia coli. Proc. Natl.     Acad. Sci. USA 85, 5879-5883, 1988. -   109. Blasi, E., Matthieson, B. J. & Varesio, L. Selective     immortalization of murine macrophages from fresh bone marrow by a     raf/myc recombinant murine retrovirus. Nature 318, 667-670, 1985. -   110. Buchner, J., Pastan, I. & Brinkmann, U. A method for increasing     the yield of properly folded recombinant fusion proteins:     Single-chain immunotoxins from renaturation of bacterial inclusion     bodies. Analytical Biochem. 205, 263-270, 1992. -   111. Kwak, L. W., Young, H. A., Pennington, R. W., & Weeks, S. W.     Vaccination with syngeneic, lymphoma-derived immunoglobulin idiotype     combined with granulocyte/macrophage colony-stimulating factor     primes mice for a protective T-cell response. Proc. Natl. Acad. Sci.     USA 93, 10972-10977, 1996. -   112. Falk, W., Goodwin, R. H., & Leonard, E. J. A 48-well micro     chemotaxis assembly for rapid and accurate measurement of leukocyte     migration. J. Immunol. Methods 33, 239-247, 1980. -   113. Solari, R., Offord, R. E., Remy, S., Aubry, J. P., Wells, T. N.     C., Whitehorn, E., Oung, T., & Proudfoot, A. B. I. Receptor-mediated     endocytosis of CC-chemokines. J. Biol. Chem. 272, 9617-9620, 1997. -   114. Feltquate, D. M., Heaney, S., Webster, R. G., & Robinson, H. L.     Different T helper cell types and antibody isotypes generated by     saline and gene gun DNA immunization. J. Immunol. 158, 2278-2284,     1997. -   115. Kwak, L. W., Campbell, M. J., Czerwinski, D. K., Hart, S.,     Miller, R. A., & Levy, R. Induction of immune responses in patients     with B-cell lymphoma against the surface-immunoglobulin idiotype     expressed by their tumors. N. Engl. J. Med. 327, 1209-1215, 1992. -   116. Kaminski, M. S., Kitamura, K., Maloney, D. G. & Levy, R.     Idiotype vaccination against murine B cell lymphoma, inhibition of     tumor immunity by free idiotype protein. J. Immunol. 138, 1289-1296,     1987. -   117. Stevenson, G. T. & Stevenson, F. K. Antibody to a     molecularly-defined antigen confined to a tumor cell surface. Nature     254, 714-716, 1975. -   118. Xu, L. L., McVicar, D. W., Ben-Baruch, A., Kuhns, D. B.,     Johnston, J., Oppenheim, J. J. & Wang, J. M. Monocyte chemotactic     protein-3 (MCP3) interacts with multiple leukocyte receptors:     binding and signaling of MCP3 through shared as well as unique     receptors on monocytes and neutrophils. Eur. J. Immunol. 25,     2612-2617, 1995. -   119. Gong, J. H., Uguccioni, M., Dewed, B., Baggiolini, M. &     Clark-Lewis, I. RANTES and MCP-3 antagonists bind multiple chemokine     receptors. J. Biol. Chem. 271; 10521-10527, 1996. -   120. Clore et al. 1990. -   121. Lodi et al. 1994. -   122. Skelton et al. 1995. -   123. Fairbrother et al. 1994 -   124. Horuk R, 1996. -   125. Bergman and Haimovich, 1977. Characterization of a     carcinogen-induced murine B lymphocyte cell line of C3H/eB origin.     Eur. J. Immunol. 7:413-417. -   126. Emini et al. 1992. Prevention of HIV-1 infection in chimpanzees     by gp120 V3 domain-specific monoclonal antibody. Nature,     355:728-730. -   127. Yarchoan et al. 1990. The National Cancer Institute Phase I     Study of 2′,3′-Dideoxyinosine Administration in Adults with AIDS or     AIDS-related Complex: Analysis of Activity and Toxicity Profiles.     Reviews of Infectious Diseases, 12(5):S522-S533. -   128. Lalani et al. (2000) Immunology Today 21:100-106. -   129. Stine et al. (2000) Blood 15:1151-1157. 

1. A fusion polypeptide comprising a viral chemokine and a human tumor antigen, wherein the viral chemokine comprises MC148.
 2. The fusion polypeptide of claim 1, wherein the human tumor antigen comprises a B cell tumor antigen.
 3. The fusion polypeptide of claim 2, wherein the B cell tumor antigen is selected from the group consisting of: (1) an antibody produced by a B cell tumor; (2) a single chain antibody comprising linked VH and VL domains which retain the conformation and specific binding activity of the native idiotype of the antibody produced by a B cell tumor; and (3) an epitope of an idiotype of an antibody produced by a B cell tumor.
 4. The fusion polypeptide of claim 3, wherein the B cell tumor antigen comprises sFv38.
 5. The fusion polypeptide of claim 1, wherein the human tumor antigen comprises gp100.
 6. The fusion polypeptide of claim 1, wherein the human tumor antigen comprises Muc-1.
 7. The fusion polypeptide of claim 1, wherein the human tumor antigen comprises the amino acid sequence of SEQ ID NO:
 1. 8. A composition comprising the fusion polypeptide of claim 1 in a pharmaceutically acceptable carrier.
 9. A method of producing an immune response in a subject, comprising administering to the subject the composition of claim
 8. 10. The method of claim 9, wherein the immune response is an effector T cell immune response.
 11. The method of claim 9, wherein the subject has a tumor.
 12. The method of claim 11, wherein the tumor is a B cell tumor.
 13. The method of claim 12, wherein the human tumor antigen is a B cell tumor antigen.
 14. The method of claim 13, wherein the B cell tumor antigen is selected from the group consisting of: (1) an antibody produced by a B cell tumor; (2) a single chain antibody comprising linked VH and VL domains which retain the conformation and specific binding activity of the native idiotype of the antibody produced by a B cell tumor; and (3) an epitope of an idiotype of an antibody produced by a B cell tumor.
 15. The method of claim 13, wherein the B cell tumor antigen comprises sFv38. 